POLYVALENT CONJUGATE VACCINE FOR CANCER

Throughout this application, various references are referred to. Disclosures of these publications in their entireties are hereby incorporated by reference into this application to more fully describe the state of the art to which this invention pertains.

BACKGROUND OF THE INVENTION

Tumor-specific antigens have been identified and pursued as targets for vaccines. Previous work from the inventors' has shown that monovalent vaccines utilizing the tumor antigens Globo H, Lewis^y, GM2, glycosylated MUC-1, Tn(c), sTn(c), or TF(c) conjugated to KLH to be safe with local erythema and edema but minimal systemic toxicities. As a result of vaccination with these monovalent vaccines, most patients generated specific high titer IgM or IgG antibodies against the respective antigen-KLH conjugates. The present invention provides a polyvalent vaccine wherein the components of the monovalent vaccines are combined and administered with an adjuvant as treatment for cancer.

SUMMARY OF THE INVENTION

The invention disclosed herein provides a polyvalent vaccine comprising at least two conjugated antigens selected from a group containing glycolipid antigen, polysaccharide antigen, mucin antigen, glycosylated mucin antigen and an appropriate adjuvant. This invention also provides the multivalent vaccine, comprising glycosylated MUC-1-32mer, Globo H, GM2, Le^y, Tn(c), and TF(c). This vaccine may comprise glycosylated MUC-1-G5, Globo H, GM2, Le^y, Tn(c), sTN(c), and TF(c). This invention provides the vaccine above, wherein the adjuvant is saponin-based adjuvant.

This invention also provides a method for inducing immune response in a subject comprising administering an effective amount of the vaccine above to the subject. Finally, this invention provides a method for treating cancer in a subject comprising administering an appropriate amount of the vaccine above to the subject.

DETAILED DESCRIPTION OF THE INVENTION

The glycolipid includes but is not limited to Globo H, a Lewis antigen and a ganglioside. The Lewis antigen includes but is not limited to Le^yand sialyl Le^a. The ganglioside includes fucosylated GM1, GM2, GD2, or GD3. In another embodiment, the mucin is a MUC peptide. In a further embodiment, the MUC peptide is MUC-1, MUC-2 or MUC-16. The polysaccharide antigen includes but is not limited to Tn(c), sTn(c), TF(c), and polysialic acid.

This invention provides a bivalent, trivalent, tetravalent, pentavalent, hexavalent, and heptavalent vaccine. The vaccine comprises at least two conjugated antigens selected from a group containing glycolipid antigen, polysaccharide antigen, mucin antigen, glycosylated mucin antigen and an appropriate adjuvant.

In an embodiment, the hexavalent vaccine comprises glycosylated MUC-1-32mer, Globo H, GM2, Le^y, Tn(c), and TF(c). In a further embodiment, the range of MUC-1-32mer is from about 0.1 to 30 ug. In yet another embodiment, the range of Globo H is from about 0.1 to 100 ug. In still a further embodiment, the range of GM2 is from about 0.1 to 100 ug. In an additional embodiment, the range of Le^yis from about 0.1 to 60 ug. In a further embodiment, the range of Tn(c) is from about 0.1 to 100 ug. In an additional embodiment, the range of TF(c) is from about 0.1 to 30 ug.

In a separate embodiment, the adjuvant is saponin based. The adjuvant includes QS21 and GPI-0100. In an embodiment, the range of QS21 is from about 25 to about 200 ug. In another embodiment, QS21 is about 100 ug. In a separate embodiment, the adjuvant is GPI-0100 with a range from about 1 to 25 mg. In an embodiment, GPI-0100 is about 10 mg.

This invention provides a heptavalent vaccine comprising at least two conjugated antigens selected from a group containing glycolipid antigen, polysaccharide antigen, mucin antigen, and glycosylated mucin antigen and an appropriate adjuvant. In an embodiment, the vaccine comprises glycosylated MUC-1-G5, Globo H, GM2, Le^y, Tn(c), sTN(c), and TF(c). In another embodiment, the range of MUC-1-G5 is from about 0.1 to 30 ug. In a further embodiment, the range of Globo H is from about 0.1 to 100 ug. In another embodiment, the range of GM2 is from about 0.1 to 100 ug. In still another embodiment, the range of Le^yis from about 0.1 to 60 ug. In an embodiment, the range of Tn(c) is from about 0.1 to 100 ug. In a further embodiment, the range of sTn(c) is from about 0.1 to 100 ug. In yet another embodiment, the range of TF(c) is from about 0.1 to 30 ug.

This invention provides the vaccine above, wherein the adjuvant is saponin-based adjuvant. These saponin-based adjuvants include but are not limited to QS21 and GPI-0100.

In an embodiment, the range of QS21 is from about 25 to 200 ug. In another embodiment, the QS21 is about 100 ug. In a separate embodiment, the adjuvant is GPI-0100 and the range is from about 1 to 25 mg. In a preferred embodiment, GPI-0100 is about 10 mg.

This invention provides a polyvalent vaccine comprising a conjugated glycosylated antigen, a conjugated ganglioside antigen and an appropriate adjuvant, wherein the antigens are conjugated to a carrier. In an embodiment, the carrier is Keyhole Limpet Hemocyanin (KLH).

This invention provides the polyvalent vaccine above comprising at least two conjugated antigens selected from a group containing glycolipid antigen, polysaccharide antigen, mucin antigen, and glycosylated mucin antigen and an appropriate adjuvant for cancer. In an embodiment, the cancer is prostate, breast or ovarian cancer.

This invention also provides a method for inducing immune response in a subject comprising administering an effective amount of the above vaccine to the subject.

Furthermore, this invention provides a method for treating cancer in a subject comprising administering an appropriate amount of the above vaccine to the subject.

This invention also provides a composition comprising the above vaccine and a carrier.

This invention also provides a pharmaceutical composition comprising the above vaccine and a pharmaceutically acceptable carrier.

In addition, the invention provides a vaccine for small cell lung cancer comprising at least two conjugated antigens selected from the group containing Globo H, fucosylated GM1, GM2, GD2, GD3, sialyl Le^aand polysialic acid. This invention also provides a method for inducing immune response in a subject bearing small cell lung cancer comprising administering an effective amount of the above vaccine to the subject. This invention furthermore provides a method for treating a subject bearing small cell lung cancer comprising administering an effective amount of the above vaccine to the subject.

In addition, this invention provides the above vaccine, further comprising an antigen selected from a group containing CA125, or a portion thereof, KSA peptide or protein, and PSMA, or a portion thereof.

This invention includes the above vaccines which further comprise other antigens which can induce antibody and/or immune response. As illustrated throughout the specification, the antigen used may be modified to increase its immunogenicity. Said antigens include but are not limited to CA125, or a portion thereof, KSA peptide or protein, and PSMA, or a portion thereof. As can be easily appreciated by the ordinary skilled artisan, only a portion of the antigen may be required for induction of immune response from a subject.

As stated herein, subjects are organisms which have immune response. The subject includes but is not limited to humans. Said subject could be domestic animals, such as dogs and cats.

This invention further provides the above compositions and a pharmaceutically acceptable carrier, thereby forming pharmaceutical compositions.

This invention also provides a pharmaceutical composition comprising a combination as described above and a pharmaceutically acceptable carrier. For the purposes of this invention, “pharmaceutically acceptable carriers” means any of the standard pharmaceutical carriers. Examples of suitable carriers are well known in the art and may include, but are not limited to, any of the standard pharmaceutical carriers such as a phosphate buffered saline solution and various wetting agents. Other carriers may include additives used in tablets, granules and capsules, etc. Typically such carriers contain excipients such as starch, milk, sugar, certain types of clay, gelatin, stearic acid or salts thereof, magnesium or calcium stearate, talc, vegetable fats or oils, gum, glycols or other known excipients. Such carriers may also include flavor and color additives or other ingredients. Compositions comprising such carriers are formulated by well-known conventional methods.

The invention will be better understood by reference to the Experimental Details which follow, but those skilled in the art will readily appreciate that the specific experiments detailed are only illustrative, and are not meant to limit the invention as described herein, which is defined by the claims which follow thereafter.

Experimental Details
First Series of Experiments
Polyvalent (Hexavalent) Conjugate Vaccine for Prostate, Breast, Ovarian and Small Cell Lung Cancer

Tumor-specific antigens have been identified and pursued as targets for vaccines. The inventors' previous work has shown that monovalent vaccines utilizing the tumor antigens Globo H, Lewis^y, GM2, glycosylated MUC-1, Tn(c), or TF(c) conjugated to KLH to be safe with local erythema and edema but minimal systemic toxicities. As a result of vaccination with these monovalent vaccines, most patients generated specific high titer IgM or IgG antibodies against the respective antigen-KLH conjugates. The present invention provides a hexavalent vaccine wherein the components of the monovalent vaccines are combined and administered with an adjuvant as treatment for prostate, breast, ovarian and small cell lung cancer.

A vaccine consisting of a unique combination of six tumor antigens administered with a saponin immunological adjuvant QS-21 or GPI-0100. The antigens are glycosylated MUC-1-32mer, Globo H, GM2, Le^y, Tn(c), and TF(c). In each case the antigen is conjugated to Keyhole Limpet Hemocyanin (KLH).

The preferred ranges of the antigen and adjuvant doses are as follows:

- Glycosylated MUC-1-32mer: 0.1 to 30 μg;
- Globo H: 0.1 to 100 μg;
- GM2: 0.1 to 100 μg;
- Le^y: 0.1 to 60 μg;
- Tn(c): 0.1 to 10 μg;
- TF(c): 0.1 to 30 μg;
- QS-21: 100 μg;
- GPI-0100: 1 or 25 mg.

Example 1
A Phase I Multivalent Conjugate Vaccine Trial for Patients with Biochemically Relapsed Prostate Cancer
1.0 PROTOCOL SUMMARY
2.0 OBJECTIVE
3.0 BACKGROUND AND RATIONALE
4.0 VACCINE PREPARATION
5.0 IMMUNIZATION SCHEDULE
6.0 PRE- AND POST-THERAPY EVALUATION
7.0 RESPONSE CRITERIA
8.0 BIOSTATISTICAL CONSIDERATIONS
9.0 REFERENCES
1.0 PROTOCOL SUMMARY

This is a phase I pilot trial designed to assess safety using a multivalent conjugate vaccine. This trial is based on the results of eight dose-seeking phase I monovalent glycoprotein and carbohydrate conjugate vaccine trials which have been shown to be consistently immunogenic in man. These trails also allowed us to screen candidate antigens for their ability to generate high titer specific antibodies against the immunizing antigen. This vaccine will consist of the highest dose of synthetic glycoprotein and carbohydrate antigens shown to elicit high titer IgM and IgG antibodies in patients with biochemically relapsed prostate cancer. The inventors' previous work has shown the monovalent vaccines to be safe with local erythema and edema but minimal systemic toxicities. Among the antigens to be included in the multivalent vaccine are carbohydrate antigens Globo H and GM2 and the glycoprotein antigens glycosylated MUC-1-32mer, Lewisy, Tn(c), and TF(c). The patient populations to be targeted are those patients who have failed primary therapies such as prostatectomy or radiation or have been on intermittent hormonal therapy and have remained hormonally sensitive in the absence of radiographic disease. These populations must have as the sole indication of disease progression, a rising PSA. The inventors' data from approximately 160 men who participated in earlier monovalent vaccine trials against the aforementioned antigens have shown that a treatment effect in the form of a decline in PSA log slopes compared with pretreatment values could be seen in patients with minimal tumor burden. A phase III double blind randomized trial with two hundred forty patients is planned based on the safety data accrued form this proposed phase I trial. The primary endpoint of the study will be the ability to assess the safety of the vaccine and the humoral response to a multivalent conjugate. Secondary endpoints will be to evaluate post-therapy changes in PSA.

2.0 OBJECTIVES
2.1 The Primary Endpoints of the Study are:

2.1.1 To determine the safety of a multivalent conjugate vaccine in patients with prostate cancer who have biochemically relapsed following primary therapies such as surgery or radiation.

2.1.2 Measure the antibody response against the individual components of the vaccine and to correlate the response to subsequent clinical course.

2.2. The secondary endpoints will be:

2.2.1 To assess post-immunization changes in prostate specific antigen levels and other objective parameters of disease (radionuclide bone scan and/or measurable disease if present.

3.0 BACKGROUND AND RATIONALE
3.1 Prostate Cancer:

Over 180,000 cases of prostate cancer will be diagnosed in the United States in 2000.¹Of these, 30-35% will present with tumors beyond the confines of the gland, while an additional 25% will develop metastases in the course of the disease despite local therapies. In these cases, a rising PSA antedates the development of overt metastases by a median of 12-24 months. Androgen ablation is the standard treatment with upwards of 70% of cases showing a normalization of an abnormal PSA after therapy. When to initiate treatment remains an area of controversy and there is no evidence that deferring therapy compromises outcomes. This observation, coupled with the fact that most patients relapsed within a median of 12-18 months², and that most men can not tolerate the side effects of castration including impotency, weight gain and hot flashes, has led to the search for alternative therapies. One such approach involves enhancing the body's own immune system as a means to treat local disease and prevent disease progression. PSA monitoring allows the identification of patients with low-volume disease, in whom an immunostimulatory approach may be more efficacious relative to a heavily pretreated, symptomatic population with large tumor burdens. Vaccinations represent a safe intervention with minimal toxicities that can be given as an adjuvant to surgery or radiation therapy in men at risk for systemic relapse. They can also be offered to men with minimal tumor burdens who are progressing and who are not willing to accept toxicities of hormonal therapy or chemotherapy. Because hormonal status may effect antigen expression and regulation, we propose to enroll patients with different hormone sensitivities. This will include patients who have not received hormonal therapy or have been on intermittent hormonal therapy.

3.2 PSA as an Endpoint for Clinical Trials:

The availability of serum PSA determinations provides a unique trial design for testing new therapies rapidly as changes in PSA levels over time correlate well with clinical outcomes.³This relationship holds for both hormone-naïve and hormonally relapsed disease. Once sequential elevations in PSA are documented in the setting of castrate testosterone levels, clinical symptoms develop in a median of 3-6 months. This observation justifies treatment in the setting of rising PSA values, using post-therapy changes in PSA as the outcome measure. With this design, therapeutic approaches that do not produce a defined degree of decline in PSA on multiple determinations for a defined duration (vide infra) are not evaluated further.²

3.3 Immunologic Approaches:

Augmentation of the immune response to cancer can be attempted by two basic approaches: non-specific immunopotentiation which constitutes the bulk of past and current efforts at cancer immunotherapy, and specific immunization which has not really been evaluated in the treatment of cancer but has contributed much to the control of infectious diseases. It is the knowledge of microbial antigens which has permitted the development of successful specific immunization against infections. The lack of availability of well-defined human cancer antigens, on the other hand, has prevented exploration of specific immunization in the context of cancer as it should be explored, using vaccines of defined cancer-restricted antigenicity and demonstrating their immunogenicity in cancer patients.

3.3.1 The Role of Carbohydrates and Mucins in Prostate Cancer:

Carbohydrate antigens have proven to be clinically relevant and (aside from vaccines against toxins) are the only defined bacterial antigens used in vaccines against bacterial pathogens. Immunization with carbohydrate antigens has also resulted in directed antibody responses against human tumor cells (reviewed in ⁴), presumably because these antibodies are known to mediate antibody-dependent cell-mediated and complement mediated lysis of tumor cells, complement-induced inflammation, and phagocytosis by the reticulo-endothelial system. The inventors' previous study in prostate cancer focused on defining the antigens expressed on the surface of prostate cancer cells.

3.3.2 Results with Eight Monovalent Phase I Trials Using Glycoprotein Peptides and Carbohydrate Antigens.

Immunohistochemistry using well-defined monoclonal antibodies against glycoprotein and carbohydrate antigens have shown that primary and metastatic prostate carcinoma specimens express these heretofore unknown antigens and that these molecules can serve as targets for immune recognition. We have studied two mucin peptide antigens, MUC-1 and MUC-2 conjugated to KLH and given with the immune adjuvant, QS21 in the phase I setting as a dose escalating trial with 10, 30 100 and 3 μg. Patients received five subcutaneous vaccines over the course of twenty-six weeks at weeks 1,2, 3, 7, and 19. Twenty patients were treated in the MUC-1-KLH-QS21 trial and fifteen were treated with MUC-2-KLH-QS21 trial. All patients developed high titer IgM and IgG antibodies specific for the immunizing peptide. Antibody titers rose by week 7 and declined usually by week 19, the time of the fifth and final vaccine. Unexpectedly, a treatment effect was observed after the vaccine trial was completed in the form of a declining PSA log slope compared with pretreatment values in approximately two-thirds of patients. In many patients, the slope began to show a decline by week 38 with subsequent declines by week 60. The initial decline corresponded to the rise of antibodies following the last immunization received at week 19. Five patients who were treated with the MUC-1-KLH conjugate in 1996 continue to have stable PSA log slopes without radiographic evidence of disease. Patients who were treated with MUC-2-KLH conjugate also demonstrated a similar treatment effect, however, the trial has not as yet reached maturity. The vaccines were found to be safe with erythema, tenderness and edema at the injection site. No evidence of autoimmunity or systemic toxicity was observed.

3.3.3 Experience with Glycolipid and Carbohydrate Antigens.

Eighteen patients have undergone immunization with Globo H, a glycolipid antigen expressed on prostate cancer cells. This is the first purely synthetic complex carbohydrate antigen used for immunization in man capable of generating high titer specific antibodies (median peak titer 1:320, IgG median titer 160) capable of mediating complement lysis of tumor cells. Several patients generated IgM antibody titers of 1:20,480). Patients were immunized with 10, 30 100 or 3 μg of Globo H-KLH plus QS21 over twenty-six weeks. Of the patients immunized with this vaccine, six remain active with stable PSA log slopes and no radiological evidence of evidence of disease over the last 2½ years. This vaccine was found to be safe with no evidence of systemic toxicity. Ganglioside antigens (acidic glycosphingolipids expressing sialic acid at one end and ceramide at the other) was also investigated in a trial comparing the immunogenicity of higher doses of QS21. Using GM2-KLH at 30 μg, a dose previously established in melanoma trials, 18 patients were immunized with either the GM2 conjugate plus QS21 at the standard dose of 100 μg or QS21 at 225 μg. Because of its potential for systemic toxicity, the latter vaccine was given as three separate immunizations to three separate sites as GM2-KLH at 10 μg plus QS21 at 75 μg subcutaneously. No difference in antibody titers were observed in two groups of patients; although two patients from the group given the higher dose of QS21 experienced grade II myalgias. Several patients also exhibited a decline in PSA log slopes but there did not appear to be any difference between groups with regard to treatment effects.

4.0 VACCINE PREPARATION

Globo H, Lewis^y, Tn(c), TF(c) are synthesized in the laboratory of Bio-Organic Chemistry headed by Dr. Samuel Danishefsky. MUC-1-32mer is synthesized in the Core Peptide Synthesis Facility of The Rockefeller Research Laboratories under the aegis of Dr. Paul Tempst. It is glycosylated with Tn by Dr. Henrik Clausen at the University of Copenhagen, Copenhagen, Denmark. GM2 is extracted from rabbit brains by Progenics, Inc., Tarrytown, N.Y.

4.1 Globo H, MUC-1-32mer, GM2, Lewis^y, Tn(c) and TF(c)-KLH Conjugation:

The above antigens will be covalently attached to KLH in Dr. Livingston's laboratory. Antigen-KLH ratios between 150/1 and 800/1 assuming a KLH molecular weight of 5×10⁶will be accepted. Gels will be performed and western blot analysis will be conducted with each lot of antigen-KLH for comparison to future lots. Sterility and safety testing with each lot plus QS21, at >50 times the dose/meter²to be used in clinical trials will be performed. No growth in culture and no adverse reaction in mice or Guinea pigs (including weight loss of 10% or more) will be tolerated. Two or more mice will be immunized with each antigen-KLH batch on 2-3 occasions at 1-2 week intervals and post immunization sera tested. Antibody titers of 1/200 or greater against antigen and 1/40 by IA or FACS staining of >25% of antigen positive cells will be accepted as proof that the construct has the appropriate immunogenicity.

4.2 Antigen Doses:

Based on previous vaccine trials in prostate cancer patients, the following doses have been established for the multivalent trial: glycosylated MUC-1-32mer, 3 μg; Globo H, 10 μg; GM2, 10 μg; Le^y, 10 μg; Tn(c), 3 μg; and TF(c), 3 μg. QS21 will be used at 100 μg as no significant difference in immunogenicity was observed with doses as high as 225 μg.

4.3 Safety Testing:

Samples from the materials are sent for sterility and safety testing. Immunogenicity of the individual peptides/carbohydrates have been previously confirmed in mice.

5.0 IMMUNIZATION SCHEDULE
5.1 Patient Selection:

All patients with evidence of biochemical relapse will be considered. Hormonal status will be recorded on the basis of serum testosterone levels as follows: Patients who have progressed after primary surgery or radiation (with or without neo-adjuvant androgen ablation) who have non-castrate levels of testosterone (>50 ng/ml) will be eligible.

5.2 Interval:

The immunization schedule that we will utilize was derived from the inventors' studies with other glycoprotein and carbohydrate conjugate vaccines in patients with melanoma, colon and breast cancers.

5.3 Treatment Schedule and Dose:

Fifteen patients will be treated with specified doses of each carbohydrate or peptide constituent as has been determined previously based on earlier monovalent trials completed. QS21 will be administered at the standard dose of 100 ug. Sites: The vaccine conjugate will be administered subcutaneously to random sites on the upper arms and upper legs.

5.4 Dose Modifications:

If a patient experiences a Grade III or greater local or Grade II or greater systemic toxicity at any time a decrease by 50% in all components of future vaccinations will be administered for that patient.

6.0 PRE- AND POST-THERAPY EVALUATION
6.1 Outcomes:

The study evaluation will include parameters to assess the safety of the vaccine, antitumor effect, as well as assessments of immune function. Interval safety assessments will include the Patient Diary. An overall antitumor assessment will be performed during weeks 13 and 26. If the patient has not demonstrated progression of disease at week 13 or 26, he will continue on protocol. Upon completion of the trial, he will be monitored every 3 months with bloodwork and imaging studies for the next 2 years or until disease progression.

6.2 Safety and Antitumor Effects:

STUDY WEEK
O^{a, c}
1
2
3
7
9
13
19
26

Clinical:

Performance Status
X^b
—
—
X
X
X
X
X
X^h

Interval Hx & PE
X^b
—
—
X
X
X
X
—
X

CBC, Diff, Plt.
X
—
—
X
X
—
X
—
X

CMP^d, LDH
X
—
—
X
—
—
X
—
X

Uric acid, Phosphorus
X
—
—
X
—
—
X
—
X

Prothrombin time
X
—
—
—
—
—
—
—
—

PSA, Ac. Phos
X
—
—
X
X
—
X
—
X

Testosterone
X
—
—
—
—
—
—
—
—

U/A
X
—
—
X
X
X
X
—
X

Stool guaiac
X
—
—
—
X
—
—
—
X

Pathology Review^e
X
—
—
—
—
—
—
—
—

Imaging:^f

Chest X-ray
X
—
—
—
—
—
X
—
X

Bone scan
X
—
—
—
—
—
X
—
X

CT Scan or MRI
X
—
—
—
—
—
X
—
X

Overall response
—
—
—
—
—
—
X
—
X

assessments^g

Consent for Pathologic
X

Correlatesⁱ

^aBaseline studies prior to immunization.

^bWithin 7 days of the first immunization.

^cWithin 15 days of starting treatment for biochemical studies; 30 days for imaging studies. Includes total bilirubin, SGOT, LDH, Alkaline Phosphatase, Creatinine, BUN.

^dCMP Includes total bilirubin, SGOT, ALT, Sodium, Potassium, Chloride, CO₂, Calcium, Glucose, Total Protein, Abumin, Alkaline Phosphatase, Creatinine, BUN.

^ePatients will be asked to obtain tissue blocks from previous diagnostic/therapeutic procedures will be obtained and the patient's tumor evaluated for the presence of the antigens by immunohistochemistry. The presence of any antigen on paraffin material is not a criterion for entry and no biopsy procedures will be performed specifically for enrollment.

^fAbdominal and pelvic CT scans with and without contrast, chest x-ray and any other tests deemed necessary to document evaluable disease.

^gOverall response assessment includes the repetition of abnormal imaging and biochemical studies used to assess disease, and in selected cases, immune function.

^hRepeat at 3 month intervals for 2 years or until disease progression is documented.

ⁱPatients will be asked to sign a separate consent for pathologic correlative studies under IRB [90-40: Dr. H. Scher, P. I. - Molecular correlations in human prostate cancer].

6.3 Immune Function:

STUDY WEEK

0
1
2
3
7
9
13
19
26

VACCINATION*
—
1
2
3
4
—
—
5
—

B-CELL TESTING
—
1
2
3
4
5
6
7
8

*No skin tests will be performed as previous trials indicated that there is minimal or no reactivity with intradermal administration of the antigens studied.

Antibody Response:

Peripheral blood (30 cc) will be drawn prior to vaccine immediately before each vaccination, as well as weeks 9, 13, and 26 to assess B-cell function. Thereafter; blood will be drawn at 3-month intervals (up to one year from the first vaccination), or as long as detectable immunity against the antigens persist. Depending on the antibody response, additional testing involving proliferation and cloning may be performed at a later date. The patients' sera will be tested by ELISA for antibodies against purified antigens as well as a variety of cell lines expressing (or not) the antigens included in the vaccine.

7.0 RESPONSE CRITERIA

7.1 Patients without Bi-Dimensionally Measurable Disease are Evaluable by Post-Therapy Changes in PSA as Follows:

7.1.1 Complete Response (CR):

Normalization of the PSA (≦1.0 or 2.0 as defined in 4.1.1) for 3 successive evaluations at least 2 weeks apart.

7.1.2 Partial Response (PR):

Decrease in PSA value by >50% above baseline (without normalization) for 3 successive evaluations.

7.1.3 Stabilization (STAB):

Patients who do not meet the criteria for PR or PROG for at least 90 days will be considered stable.

7.1.4 Progression (PROG):

Three consecutive increases in PSA, to >50% above baseline.

7.2 Duration of Response:

Non-measurable disease: Time from initiation of therapy until a 50% increase from the PSA nadir value is documented on three successive determinations.

8.0 BIOSTATISTICAL CONSIDERATION

8.1 This is an exploratory study to study the safety of a multivalent conjugate vaccine which will be taken to phase III clinical trials. Patients with prostate cancer who have experienced a PSA recurrence after radical prostatectomy or radiation therapy are eligible. All fifteen patients will receive the same dose. The dose is based on previous vaccine trials in prostate cancer patients, the following doses have been established for the multivalent trial: glycosylated MUC-1-32mer, 3 μg; Globo H, 10 μg; GM2, 10 μg; Le^y, 10 μg; Tn(c), 3 μg; and TF(c), 3 μg. QS21 will be used at 100 μg as no significant difference in immunogenicity was observed with doses as high as 225 μg. Subjects will be followed for two years or until the development of metastatic disease. Bone scan and CT scans (or MRI where clinically appropriate) will be performed approximately at week 13, 26, and approximately every 3 months thereafter until the development of metastatic disease. In addition, PSA measurements will be obtained at weeks 3, 7, 13, 26, and every approximately 3 months thereafter in order to study the effect of the vaccine on the probability of developing metastatic disease and the effect of the vaccine on PSA slope over time, respectively.²⁴

8.2 In order to be eligible for the study, patients must have a rising PSA following radical prostatectomy or radiation therapy. This detection of PSA following treatment must occur within two years.²⁵sing the ASTRO definition, three consecutive PSA rises are considered a biochemical failure after radical prostatectomy or radiation therapy. The date of failure should be the midpoint between the postsurgical (or postirradiation) nadir PSA and the first of the three consecutive rises.²⁵In addition, patients must have a PSA doubling time (DT) less than 5 months. PSA doubling time is determined prior to treatment and is equal to ln(2) divided by the least squares derived slope of log PSA over time (log PSA slope>0.15).²⁶The time interval in which PSA DT will be based will consist of a minimum of three PSA measurements in a twelve-month interval prior to randomization. Patients who meet this requirement are considered at a higher risk for metastatic disease and will be eligible for this trial.

8.3 The primary objective of this study is to determine the safety and the humoral response of the multivalent vaccine in preparation for the phase III trial. The primary endpoint will be the time to radiographic progression of disease. The secondary objective is to study the rate of change in PSA over time.

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10. Ho S B, Niehans G A, Lyftogt C, Yan Ps, et al: Heterogeneity of mucin gene expression in normal and neoplastic tissues. Cancer Res, 53:641-651, 1993.

11. Slovin, S. F., Livingston, P., Zhang, S., Keeperman, K., Mhatre, S., Adluri, S., Ghossein, R., Glazewski, J., Gordils, J., Danishefsy, S., and Scher, H. I.: Targeted therapy in prostate cancer (PC): vaccination with a glycoprotein, MUC-1-KLH-QS21 peptide conjugate. Proc Am Soc Clin Onc., 16:311a (Abstr 1107), 1997.

12. Slovin, S. F., Livingston, P., Keeperman, K., Mhatre, S., Danishefsky, S., Glazewski, J., Adluri, S., Zhang, S., Gordils, J., and Scher, H. I.: Targeted therapy in prostate cancer: vaccination with glycoprotein, MUC-1-KLH-QS21 peptide conjugate. J. Urol., 157:160 (Abstr 620), 1997.

13. Zing P X, Apostolopoulos V, Prenzoska J, et al: Petioled binding sites recognized by anti-mucin (MUC-2) antibodies. Scand J Immun, 591-592, 1994.

14. Slovin, S. F., Ragupathi, G., Donaldson, C., Olkiewicz, K., Terry, K., DePaolo, R., Livingston, P. O, and Scher, H. I.: MUC-2-KLH conjugate vaccine: Immunogenicity in patients with relapsed prostate cancer. Proc. Amer. Assoc. Cancer Res, 40:312(Abstr #2071), 1999.

15. Ragugpathi, G., Adluri, R., Amaravathi, R., Howarad, L., Gilewski, T., Slovin S. F., and Livingston, P. O.: Specificity analysis of sera from breast and prostate cancer patients vaccinated with MUC1-KLH and MUC-2-KLH conjugate vaccines. Proc. Amer. Assoc. Cancer Res, 40:312 (Abstr #2070), 1999

16. Slovin, S. F., Livingston, P. O., Danishefsky, S., Mhatre, S., Ragupathi, R., Depaolo R., Sames, D., Terry K., Bauso, A., Kelly, W. K., Fazzari, M., and Scher, H. I.: Carbohydrate vaccines as immunotherapy for prostate cancer (PC): Globo-H-KLH conjugate plus QS21. Proc Am Soc Clin Onc, 17:433a (Abstr 1669), 1998.

17. Slovin, S F, Ragupathi G, Adluri S, Ungers G, Terry K, Kim S, Spassova M, Bornmann, W G, Fazzari M, Dantis L, Olkiewicz K, Lloyd K O, Livingston P O, Danishefsky S J, and Scher H I: Carbohydrate vaccines in cancer: Immunogenicity of a fully synthetic globo hexasaccharide conjugate in man. Proc Natl Acad Sci, USA, 96:5710-5715, 1999.

18. Slovin, S., Ragupathi, G., Israel, R., Terry, K., Bauso, A., Fazzari, M., Kelly, K., Reyes, S., Livingston, P., and Scher, H. Ganglioside vaccines in relapsed prostate cancer (PC): Experience with GM2-KLH conjugate plus the immunologic adjuvant, QS21-A trial comparing QS21 doses. Proc. Amer. Soc. Clin. Onc., 18:316 Aa(Abstr #1214), 1999.

19. Livingston P O, Natoli E J, Calves M J: Vaccines containing purified GM2 ganglioside elicit antibodies in melanoma patients. Proc natl Acad Sci USA, 27:537, 1987 (Abstract).

20. Slovin, SF, et al: Tn-cluster (c)-KLH/PAM vaccine conjugates in biochemically relapsed prostate cancer (PC): Phase I trial results. Proc. Amer. Assoc. Cancer Res, in press.

21. MacLean G D, Reddish M, Koganty, R R, Wong T, Gandhi S, Smolenski M, Samuel J, Nabholtz J M, and Longenecker B M: Immunization of breast cancer patients using a synthetic sialyl-Tn glycoconjugate plus Detox adjuvant. Cancer Immunol Immunotherap 36:215-222, 1993.

22. Zhang S, Walberg L A, Ogata S, Itzkowitz S H, Koganty R R, Reddish M, Gandhi S S, Longenecker B M, Lloyd K O and Livingston P O: Immune sera and monoclonal antibodies define two configurations for the sialyl Tn tumor antigen. Cancer Res 55:3364-3368, 1995.

23. MacLean G D, Bowen-Yacyshyn M B, Samuel J, Meikle A, Stuart G, Nation J, Poppema S, Jerry M, Koganty R, Wong T, and Longenecker B M: Active immunization of human ovarian cancer patients against a common carcinoma (Thompson-Friedenreich) determinant using a synthetic carbohydrate antigen. J Immunotherapy, 11:292-305, 1992

24. Scher, H. I, Slovin, S. F., Kelly, W. K., Livingston, P. O., Danishefsky, S., Fazzari, M., Terry, K. And Heller, Glen: Intermediate markers in assessing response to vaccine therapies. Proc Am Soc Clin Onc, 17:324a (Abstr 1247), 1998.

25. Patel, A, Dorey, F, Franklin, J, and DeKernion, J B: Recurrence patterns after radical retropubic prostatectomy: Clinical usefulness of prostate specific antigen doubling times and log slope prostate specific antigen. J Urol, 158:1441-1445, 1997.

26. O'Brien, PC, Fleming, T R: A multiple testing procedure for clinical trials. Biometrics 35:549-556, 1979.

Example 2
Hexavalent Vaccine Immunogenicity Trial in Mice Methods
Serological Analyses
1. ELISA (Enzyme-Linked ImmunoSorbent Assay):

ELISA assays were performed as described below. Antigen in ethanol or in 0.1 M carbonate buffer (pH 11) were coated on ELISA plates at 0.2 μg/well for glycolipids and 0.1 μg/well for peptides. Serially diluted antiserum was added to each well and alkaline phosphatase-conjugated goat anti-mouse IgM or anti-mouse IgG was added at a dilution of 1:200 (Southern Biotechnology Associates, Inc, Birmingham, Ala.). Goat anti-mouse IgG and IgM conjugated with alkaline phosphatase obtained from Kierkegaard and Perry Labs, (Gaithersburg, Md.) were used as second antibodies. ELISA titer is defined as the highest dilution yielding an absorbance of 0.1 or greater over that of normal control mouse sera.

2. Cell Surface Reactivity Determined by FACS:

The cell surface reactivity of immune sera was tested on human cell lines. Single cell suspensions of 2×10⁵cells/tube were washed in PBS with 3% fetal calf serum (FCS) and 0.01M NaN₃and incubated with 20 μl of 1:20 diluted sera or monoclonal antibody mAb for 30 min on ice. After two washes with 3% FCS in PBS, 20 μl of 1:15 diluted goat anti-mouse IgM or IgG-labeled with fluorescein-isothiocyanate (FITC, Southern Biotechnology Associates Inc. Birmingham, Ala.) was added, and the mixture incubated for 30 min. After a final wash, the positive population and mean fluorescence intensity of stained cells were differentiated using FACScan, Becton & Dickinson Immunocytometry, San Jose, Calif.

APPENDIX B

Hexavalent Vaccine Immunogenicity Trial in Mice

Four female CB6F1 mice were vaccinated weekly for three weeks with Hexavalent vaccine

(Hexavalent vaccine in Polyval-KLH conjugate plus 20 ug QS21 per mouse).

The injections were SC, at 2 sites, with 95 ul/site.

[Vial labeled Polyval in Polyval-KLH conjugate plus 100 ug QS21/1.0 ml. Total vol. 1.0 ml. Lot # 081100]

Pre-vaccination sera was drawn from each mouse.

Sera was drawn again at 10 days post third vaccination.

The mice were weighed prior to and post vaccination

(at 24 hr post, at 48 hr post, at one week post and at 2 weeks post).

For controls, the following monoclonal antibodies were used:

VK9
anti-Globo-H

BR96
anti-Le^y

HMFG1
anti-MUC1

αTn Ab
anti-Tn

αGM2 Ab
anti-GM2

49H.8
anti-TF

SEROLOGY

ELISA plates were coated with 0.1 ug/well of one of the following antigens: GloboH-ceramide, GM2(IgM), MUC1G5, Tn-′HSA,

Tf-′HSA

ELISA plates were coated with 0.2 ug/well of one of the following antigens: GM2 (IgG), Ley

Sera was tested at an initial dilution of 1:40, with subsequent 2-fold dilutions (with the exception of GloboH for which 3-fold

dilutions were used).

FACS analysis was performed on two cell lines: MCF7 and LSC (5 × 10⁵cells per tube).

Sera was added at a 1:20 dilution (25 ul/tube).

Each post 3rd vacc. sera was set against its corresponding pre-sera (each pre-sera was set at 10%).

Appendix B Results

ELISA

Globo H
GM2
Le^Y

IgG
IgM
IgG
IgM
IgG
IgM

Mouse #
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd

1
0
40
120
1,080
40
40
40
80
0
40
80
640

2
0
80
40
3,240
40
40
40
80
0
40
80
80

4
0
360
120
3,240
0
0
0
80
0
40
40
640

5
0
40
0
3,240
0
40
0
80
0
160
40
320

+control
VK9 1:25,600

αGM2 >>>1:1,000,000
BR96 (1 ug/ul)

1:3,200

MUC1G5
Tf-′HSA
Tn-′HSA

IgG
IgM
IgG
IgM
IgG
IgM

Mouse #
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd
presera
post 3rd

1
0
10,240
0
80
0
640
0
80
0
1,280
0
80

2
0
20,480
0
320
0
640
0
160
0
640
0
5,120

4
0
5,120
0
40
0
5,120
0
160
0
10,240
0
640

5
0
10,240
0
160
0
10,240
0
160
0
10,240
40
640

+control

49H.8 1:1,600

aTn 1:25,600

FACS

MCF7
LSC

IgG
IgM

IgG
IgM

Mouse #
presera
post 3rd
presera
post 3rd
+controls

presera
post 3rd
presera
post 3rd
+controls

1
10.02%
95.76%
11.52%
89.79%
VK9
1.13%
10.11%
42.28%
9.63%
58.23%
VK9
0.95%

2
10.49%
95.30%
10.48%
95.61%
BR96
97.11%
9.60%
28.88%
10.75%
93.47%
BR96
94.85%

4
9.78%
94.71%
11.36%
95.96%
HMFG1
62.31%
9.93%
27.09%
11.12%
96.28%
HMFG1
1.19%

5
9.78%
95.48%
9.86%
94.49%
αTn Ab
78.62%
10.59%
23.46%
10.16%
93.23%
αTn Ab
57.63%

2⁰Ab alone

1.28%

1.15%
αGM2 Ab
94.91%

1.18%

1.14%
αGM2 Ab
63.94%

49H.8
0.14%

49H.8
0.26%

Second Series of Experiments
Polyvalent (Heptavalent) Conjugate Vaccine for Prostate, Breast, Ovarian and Small Cell Lung Cancer

Tumor-specific antigens have been identified and pursued as targets for vaccines. The inventors' previous work has shown that monovalent vaccines utilizing the tumor antigens Globo H, Lewis^y, GM2, glycosylated MUC-1, Tn(c), sTn(c), or TF(c) conjugated to KLH to be safe with local erythema and edema but minimal systemic toxicities. As a result of vaccination with these monovalent vaccines, most patients generated specific high titer IgM or IgG antibodies against the respective antigen-KLH conjugates. The present invention provides a heptavalent vaccine wherein the components of the monovalent vaccines are combined and administered with an adjuvant as treatment for prostate, breast, ovarian and small cell lung cancer.

A vaccine consisting of a unique combination of seven tumor antigens administered with a saponin immunological adjuvant QS-21 or GPI-0100. The antigens are glycosylated MUC-1-G5, Globo H, GM2, Le^y, Tn(c), sTn(c), and TF(c). In each case the antigen is conjugated to Keyhole Limpet Hemocyanin (KLH).

The preferred ranges of the antigen and adjuvant doses are as follows:

Glycosylated MUC-1-G5: 0.1 to 30 μg;

Globo H: 0.1 to 100 μg;

GM2: 0.1 to 100 μg;

Le^y: 0.1 to 60 μg;

Tn(c): 0.1 to 100 μg;

sTn(c): 0.1 to 100 μg;

TF(c): 0.1 to 30 μg;

QS-21: 25-200 μg;

GPI-0100: 1-25 mg.

Example 1

Phase I clinical trial protocol using the heptavalent vaccine

Example 2

Heptavalent vaccine immunogenicity trial in mice

1. Methods

2. Results

Example 1
Pilot Phase I Trial in Patients with Epithelial Ovarian, Fallopian Tube, or Peritoneal Cancer with a Polyvalent Vaccine-KLH Conjugate+Qs-21
1.0 PROTOCOL SUMMARY
2.0 OBJECTIVE
3.0 BACKGROUND AND RATIONALE
4.0 VACCINE PREPARATION
5.0 TREATMENT SCHEDULE AND DOSE
6.0 EVALUATION DURING STUDY
7.0 BIOSTATISTICAL CONSIDERATIONS (Endpoints)
8.0 BIBLIOGRAPHY
1.0 PROTOCOL SUMMARY AND PROGRAM PLAN

Patients with epithelial ovarian, fallopian tube, or peritoneal cancer who receive surgical cytoreduction and platinum/taxane containing chemotherapy have a significant chance of entering complete clinical remission but unfortunately approximately 70% will eventually relapse. These patients in clinical remission have minimal residual disease, and are excellent candidates in which to evaluate novel consolidation strategies in an attempt to improve outcome. This pilot polyvalent protocol represents the culmination of a series of monovalent phase I vaccine trials at the center demonstrating the immunogenicity of the various component antigens. It represents the transition between the phase I monovalent trial program in second remission, to the planned development of larger trials designed to evaluate efficacy. Immunization with the individual antigens selected for this vaccine has been consistently immunogenic in the majority of patients. No confirmed systemic toxicity has occurred related to vaccine administration. It is expected that the immunogenicity will remain unchanged, and that no systemic toxicity will occur with polyvalent vaccine administration. Eligible patients for this pilot trial are those patients initially with stage II-IV disease in complete clinical remission following primary therapy, or following relapse and re-induction to remission with additional chemotherapy. In this trial, patients will receive an antigen defined vaccine with the following ganglioside components: a) GM2, b) Globo-H; the blood group related antigens: c) TF(c), d) s-Tn (c), e) Tn (c) f) Lewis-Y; and g) the protein antigen MUC-1-G5 (glycosylated). The primary endpoints of this pilot study are safety, and confirmation of continued immunogenicity. The secondary endpoint will be to characterize the nature and duration of the antibody response.

2.0 OBJECTIVES

2.1 The primary endpoints of this pilot study are to determine the safety of polyvalent vaccine administration, and continued immunogenicity in patients prior to conducting a large, randomized study.

2.2.2 The secondary endpoint is to further characterize the nature and duration of the antibody response generated by the polyvalent vaccine (ELISA and FACS)

3.0 BACKGROUND AND RATIONALE
3.1 Disease Background and Suitability for Treatment

In 1999, approximately 22,500 new cases of ovarian cancer were diagnosed, and it is estimated that 14,500 women died of the disease. Seventy-five percent of patients with ovarian cancer will have spread beyond the ovary at diagnosis. Standard primary treatment consists of cytoreductive surgery followed by a platinum and paclitaxel containing chemotherapy regimen.¹Many patients have no clinically measurable disease at the end of primary treatment. A review of second-look laparotomy, however, indicates that less than 50% of patients are actually free of disease.²Furthermore, nearly half of patients with a negative second look procedure are destined to relapse and require additional treatment.^3,4Overall, only approximately 30% of patients remain disease free with currently available treatment. Given the minimal disease burden at the completion of primary therapy, these patients are ideal candidates in which to evaluate immune modulating strategies.

3.2 Rationale for Polyvalent Vaccines Designed Primarily for Antibody Production

Varied data exists in solid tumors to support the development of immune directed therapy. Studies have emerged in patients with melanoma which demonstrate that naturally acquired ^5,6, or actively induced ^7,8antibodies may improve outcome. In a large clinical trial reported by Reithmuller et al., 189 patients with resected Dukes C colon carcinoma were randomized to receive observation versus postoperative treatment with murine antibody CO17-1A that recognizes the KSA antigen. Toxic effects were limited to infrequent constitutional symptoms. At median follow-up of five years, the death rate was 36% in the treated group versus 51% in the observed group. The advantage of treatment was demonstrated in univariate (p=0.051) and multivariate (p=0.043) analysis when controlling for other known prognostic factors.⁹

The basis for cancer vaccines designed primarily for antibody induction are the many preclinical models demonstrating the ability of passively administered or actively induced antibodies to prevent tumor recurrence the increasing number of clinical trials where passively administered monoclonal antibodies have demonstrated clinical efficacy, and the correlation of antibodies, naturally acquired or vaccine induced, with improved prognosis in several different clinical settings.⁶

EL4 lymphoma naturally expresses GD2 ganglioside, which is recognized by monoclonal antibody 3F8. Vaccines containing GD2 covalently conjugated to KLH and mixed with immunological adjuvant QS21 are the optimal approach to vaccination against GD2. Relatively higher levels of antibody administered two or four days after intravenous tumor challenge or moderate titers induced by vaccine that were present by day two or four after tumor challenge were able to eradicate disease in most mice. If antibody administration was deferred until day seven or ten, little or no benefit could be demonstrated. If the number of cells in the EL4 challenge was decreased, giving a longer window of opportunity, the vaccinations could be initiated after tumor challenge and good protection seen.⁷These results are consistent with the need to initiate immunization with vaccines inducing antibodies in the adjuvant setting, when the targets are circulating tumor cells and micrometastases. Patients with ovarian cancer in first remission meet these criteria, and unfortunately have a high “event rate” (ie. 80% will relapse) allowing for the rapid assessment of the efficacy of this approach.

The basis for the inventors' emphasis on polyvalent vaccines is tumor cell heterogeneity, heterogeneity of the human immune response and the correlation between overall antibody titer against tumor cells and effector mechanisms such as complement mediated cytotoxicity (CDC) or antibody dependent cell mediated cytotoxicity (ADCC). For example, using a series of 14 tumor cell lines and monoclonal antibodies (mAbs) against 3 gangliosides, investigators at MSKCC have shown that significant cell surface reactivity analyzed by flow cytometry and CDC increased from 2-8 of the cell lines using one of three mAbs to 13-14 of the cell lines when the 3 mAbs were pooled. The median CDC increased 4 fold with the pool of mAbs compared to the best single mAbs.¹¹Cancers of the ovary express a rich array of cell surface antigens making them especially suitable targets for polyvalent vaccines.

Cell surface antigens (especially carbohydrate cell surface antigens) have proven to be unexpectedly potent targets for immune recognition and attack of human cancers. Many of the more tumor-restricted monoclonal antibodies derived by immunization of mice with human tumor cells have been found to be directed against carbohydrate antigens expressed at the cell surface¹²Immunization against carbohydrate antigens results generally in an antibody response (see references for dissenting views), which is primarily IgM.^13-15These antibodies are known to induce CDC, inflammation, and phagocytosis of tumor cells by the reticulo-endothelial system (opsonization).¹⁶Immunization against cell surface protein antigens can induce a variety of B and T lymphocyte responses. The T lymphocyte responses are difficult to quantify in the context of vaccination trials and are not the focus of this proposal. The antibody responses against protein antigens contain IgM and IgG, both of which can induce complement activation (with regard to IgG depending on the subclass, IgG1 and IgG3 being optimal). IgG antibodies of these subclasses can also induce ADCC.

Antibodies are the primary mechanism for active elimination of circulating pathogens from the bloodstream. They are ideally suited for eradication of free tumor cells and systemic or intraperitoneal micrometastases and they have accomplished this as described above in a variety of preclinical mouse experiments (reviewed in references).^10,7In adjuvant immunization trials, the primary targets are individual tumor cells or early micrometastases which may persist for long periods after apparent resection of all residual tumor.¹⁷After surgery and completion of chemotherapy is the ideal time for immune intervention, and in particular for administration of cancer vaccines aimed at instructing the immune system to identify and kill the few remaining cancer cells. If antibodies of sufficient titer can be induced against tumor antigens to eliminate tumor cells from the blood and lymphatic systems, aggressive local therapies, including surgery, radiation therapy and intralesional treatments might result in long term control of even metastatic cancers.

3.3 Preliminary Studies for the Antigens

GM2 vaccines: Investigators at the center have been refining the ability to induce antibodies against GM2 in melanoma patients for fifteen years, since first demonstrating that vaccines containing purified GM2 could be more immunogenic than vaccines containing tumor cells expressing GM2.¹⁸Initially GM2 adherent to BCG was selected as optimal, inducing IgM antibodies in 85% of patients. This was the basis for a randomized trial comparing immunization with BCG to immunization with GM2/BCG in 122 patients with AJCC Stage 3 melanoma.⁸The IgM antibodies had a median titer of 1/160 and were short lived (8-12 weeks). IgG antibody induction was rare. Antibody titers have been maintained for over three years by administration of repeated booster immunizations at 3-4 month intervals. When comparing patients as randomized in this trial, no statistically significant difference on overall or disease free survival was seen. Pre-existing GM2 antibodies were seen in 5 patients in the control group, as opposed to one in the GM2 treated group which may have blunted the treatment result. The association between better outcome and the presence of GM2 antibodies was seen (8).

TF, Tn and sTn Vaccines:

Patients with various epithelial cancers have been immunized with unclustered TF-KLH and sTn-KLH conjugate vaccines plus various adjuvants.¹⁹High titer IgM and IgG antibodies against TF and sTn antigens have resulted, but we found that the majority of the reactivity detected in sera from immunized mice and patients was against antigenic epitopes present on synthetic constructs which were not present on naturally expressed mucins.²⁰Based on previous studies with Tn antigen,²¹Kurosaka and Nakada et al. hypothesized that MLS102, a monoclonal antibody against sTn, might preferentially recognize clusters (C) of sTn. In studies at MSKCC with monoclonal antibody B72.3 and with sera raised against TF-KLH and sTn-KLH conjugate vaccines in mice and in patients resulted in the same conclusion.^20,22The availability of synthetic TF, Tn and sTn clusters consisting of 3 epitopes covalently linked to 3 consecutive serines or threonines has permitted investigators at MSKCC to prove this hypothesis. In both direct tests and inhibition assays, B72.3 recognized sTn clusters exclusively, and sera from mice immunized with sTn (C)-KLH reacted strongly with both natural mucins and tumor cells expressing sTn.²²Based on this background, we initiated trials with the TF(C)-KLH, Tn(C)-KLH and sTn(C)-KLH conjugate vaccines in patients with breast cancer. Antibodies of relevant high titer specificity, including against OSM or PSM and cancer cells expressing TF, Tn or sTn, have been induced for the first time in the inventors' experience. Based on these results confirming the importance of clustered epitopes and defining their relevant immunogenicity, we are including these clustered antigens in the polyvalent vaccine against ovarian cancer.

Le^yand Globo H Vaccines:

The development of Le and Globo H vaccines was previously limited by the lack of sufficient quantities of antigen for vaccine construction and testing. Over the last four years, Dr. Danishefsky has successfully synthesized both antigens.^23,24Investigators at MSKCC have immunized groups of mice with Globo H-ceramide plus or minus adjuvants QS-21 and Salmonella minnesota mutant R595, and with Globo H covalently attached to KLH or BSA plus immunological adjuvant QS-21. The highest antibody titers against both synthetic antigen and MCF7 cells expressing Globo H were induced by the Globo H-KLH plus QS-21 vaccine.^23,24The antibody titer induced against synthetic Globo H was 1/120,000 by ELISA, the titer induced against MCF7 was 1/320, and potent complement mediated cytotoxicity was seen as well. Le^y-BSA and Le^y-KLH vaccines have also been tested in the mouse. High titer antibody responses have resulted against the synthetic epitope of Le^yand against tumor cells expressing Le^yin the majority of mice immunized.²⁵Based on these results, monovalent phase I clinical trials with Globo H-KLH plus QS-21 and Le^y-KLH plus QS21 have been initiated in patients with breast, prostate or ovary cancer. Antibodies against the purified antigens and against tumor cells expressing these antigens were induced in most patients and the manuscript was recently published for the latter.^26,27

MUC1 and MUC2 Vaccines:

Investigators at MSKCC have immunized mice with MUC1-KLH and MUC2-KLH, plus QS-21, and seen induction of consistent high titer IgM and IgG antibodies against MUC1 and MUC2 and human cell lines expressing MUC1 and MUC2, as well as protection from a syngeneic mouse breast cancer expressing human MUC1 as a consequence of gene transduction. Mice were also immunized with vaccines containing MUC1 peptides of various lengths conjugated to KLH by one of three methods or not, and mixed with QS-21 or BCG. MUC1 containing 30 amino acids or more, conjugated to KLH with an MBS bifunctional linker and mixed with immunological adjuvant QS-21 induced the highest titer antibodies.²⁸Based on these studies in the mouse, a trial was initiated and completed a trial with this MUC1-KLH plus QS-21 vaccine in breast cancer patients who were free of detectable breast cancer after resection of all known disease. Nine patients were treated with a 31 amino acid MUC1 peptide with cysteine at one end for conjugation to KLH and the immune dominant epitope-APDTRPA at the other end.²⁹No patient had detectable MUC1 serological reactivity by ELISA or FACS prior to immunization. The results are summarized below in table below. Reactivity against MUC1 and tumor cells expressing MUC1 was seen in most patients. A separate group of patients were immunized with MUC2-KLH plus QS21. Analysis of this trial is not yet complete, but the results to date are also summarized in the table below.

The inventors have been unable to demonstrate T-lymphocyte proliferation, interferon γ and IL4 release by ELISPOT assays, CTL activity or positive DTH responses after vaccination with MUC1 or MUC2. The proliferation assays were particularly focussed on in the MUC1 trials. Patients had leukophoresis pre and post vaccination, providing ample lymphocytes for study. After 2 years of steady endeavor, there has been no clear evidence of augmented reactivity against MUC1 peptides of various lengths or, in HLA A2 positive patients against heteroclytic MUC1 peptides with single amino acid changes that increased binding to HLA A2. (personal communication, P. O. Livingston) Pre and post vaccination PBLs from the first 6 patients vaccinated with MUC1 were also sent to the laboratory of Dr. Olivera Finn for CTL precursor frequency analysis. No increase in frequency was seen. Over all, the major difference between results from MSKCC with the 31aa MUC1-KLH plus QS-21 vaccine and Dr. Finn's results with a 104aa MUC1 peptide plus BCG vaccine was that the former had a clearly demonstrable, consistent antibody response, which was reactive with tumor cells. Inhibition assays were performed to better understand this serologic response.³⁰Much of the IgM response and nearly all of the IgG response were against the immune dominant epitope, APDTRPA, preferentially with RPA at the terminal position.

KSA Vaccines:

KSA has been prepared in the baculovirus system by Jenner Technologies (San Ramon, Calif.) and 10 mcg/patient has been provided for testing. Due to the small quantity of KSA available, following demonstration of relevant immunogenicity in mice, we treated groups of 9 patients with KSA plus QS21 or with KSA covalently linked to KLH by glutaraldehyde, plus QS21. In neither case was there significant induction of antibodies against KSA that had not been glutaraldehyde treated, or tumor cells expressing KSA. Consequently KSA will not be included in the polyvalent vaccine. The results of this and the other trials with KLH conjugate vaccines are summarized in the table below (personal data, P. O. Livingston).

Summary of Serological Results in Vaccinated Patients

Median

Median

ELISA
IgG
FACS
Median
Median

Antigen
IgM
IgG
Subclass
IgM
IgG
IA
CDC

GM2
640
320
IgG1 + 3
+++
++
++
++

Globo H
640
40
IgG1 + 3
++
+
++
+

Lewis^y
80
0

++
+
+
+

Tn
1280
1280

++
−
+
−

STn
1280
160
IgG3
+++
−
+
−

TF
320
10

−
+
−

MUC1
1280
5120
IgG1 + 3
+
−
+
−

MUC2
2560
2560
pending

KSA
40
160

−
−
−
−

Additional Variables:

Two additional variables have proven critical, the method of conjugation and the epitope ratio of antigen molecules per KLH molecule. The optimal conjugation approached has varied with the antigen. Gangliosides are best conjugated using ozone cleavage of the ceramide double bond and introducing an aldehyde group followed by coupling to aminolysyl groups of KLH by reductive amination. This approach was not as effective for conjugation of Tn, sTn and TF clusters or Globo H to KLH where an M2C2H linker arm has proved most efficient³¹or for MUC1 or MUC2 where an MBS linker group was optimal.²⁸

The impact of dose and schedule of vaccine administration on antibody response to GM2 vaccines in melanoma patients has also been explored. Immunization 4 times at weekly intervals or biweekly intervals followed by booster immunizations twice at 2-3 month intervals was compared to 6 immunizations at monthly intervals. Initial immunizations at weekly or biweekly intervals resulted in comparable high titers (with high titers occurring slightly sooner at weekly intervals), but remarkably the monthly immunizations resulted in far weaker or undetectable antibody responses in the 6 patients vaccinated.³²GM2-KLH plus QS-21 vaccines prepared at MSKCC and at Progenics Pharmaceuticals have each been tested in dose finding studies such as those proposed in this application. In both cases GM2 doses of 3 ug or less resulted in lower IgM titers and undetectable IgG titers in most patients. GM2 doses of 10, 30 and 100 ug gave comparable IgM and IgG titers.³³Based an these studies, we have selected the initial weekly schedule of 3-4 immunizations followed by booster immunizations every three months, and the doses for use in the randomized Phase III trial.

3.4 Potential Toxicity of Vaccination

The expected safety of the vaccine is based on the safety of vaccination with the individual components. Clinical experience is growing in clinical trials with vaccine induced antibody responses against each of the included antigens. Antigen expression at secretory borders in these trials, where the majority is located, has induced neither immunological tolerance nor symptomatic autoimmunity once antibodies are present, suggesting they are sequestered from the immune system. Nevertheless, a regular schedule of laboratory studies and physical examinations are designed to detect any abnormalities. This pilot trial will represent one of the first studies to confirm the safety of polyvalent vaccine administration in this setting.

3.5 General Immune Approaches

Various methods have been used to increase the immunogenicity of antigens, and in particular for inducing an IgG response. In preclinical laboratory studies, we have found the covalent attachment of antigen to keyhole limpet hemocyanin (KLH) to be most effective.³⁴KLH is well tolerated, and has previously caused only mild inflammation at the vaccine injection site. Attachment of KLH may be accomplished by a variety of cross-linking methods. MBS (m-maleimidobenzoly-N-hydroxysuccinimide ester) is the best-known heterobifunctional reagent; and at neutral pH cross-links thiol groups with amino groups. The linkage proceeds via two separate reactions, thus limiting bonds between identical molecules. In addition to linking antigen to immunogenic carrier proteins, the titer of antibody induced may be further augmented with the use of appropriate immunological adjuvants. We have immunized groups of melanoma patients with vaccines either containing no adjuvant, or using DETOX, BCG or QS-21. QS-21 is a significantly more effective adjuvant than the others, producing significantly higher titer IgM and IgG antibodies. It is a saponin derivative extracted from the bark of the South American tree Quillaja saponaria Molina. The monosaccharide composition, molecular weight, adjuvant effect and toxicity for a series of these saponins have been described.^35-36It has also proven to be non-toxic and effective at augmenting the immunogenicity of an FeLV subunit vaccine in cats ³⁷and an HIV-1 recombinant vaccine in Rhesus monkeys. A phase I trial demonstrating the safety and suggesting the efficacy of a 100 ug QS-21 dose in patients treated with GM2-KLH vaccines has been reported. The only adverse events reported were minimal flu-like symptoms, and mild discomfort at the injection site.³⁸Thus, conjugation with KLH and the addition of QS-21 have become standard approaches for vaccine construction at MSKCC has proven optimal for antibody induction against a variety of gangliosides, MUC1, MUC2, KSA, Tn, sTn, TF, Le^yand Globo H in the mouse and in humans.

3.6 Distribution of the Antigens Studied:

In general, the antigens contained in this vaccine are expressed on ovarian cancer cells with high frequency. Recent studies at MSKCC have characterized this distribution in a variety of tumor types including ovarian cancer using immunohistochemical staining. A variety of tumor specimens were used in each tumor type, and it was required that 50% or more cells be positive in order to consider the antigen present. The presence of these antigens on the tumor specimens tested in ovarian cancer was: GM2 (100%), GLOBO-H (60%), MUC 1 (100%), sTn (60%), TF (100%), Le Y (80%).^39-41

3.7 Rational for the Inventors' Approach:

The inventors' hypothesis is that induction of an antibody response against several cell surface antigens on ovarian cancer cells with a polyvalent conjugate vaccine will result in eradication of free tumor antigen, circulating tumor cells and micrometastases. The polyvalent nature of the vaccine and antibody response is important to eliminate escape by tumor cells that fail to express any one or two of the antigens, and to increase the number of antibodies reacting against each cell. It is expected that the inventors' vaccine will prove consistently immunogenic against five or six of the ovarian cancer cell surface antigens described above, and that it will prove nontoxic. Whether immunization with this polyvalent vaccine in high-risk ovarian cancer patients in the remission setting will result in prolonged disease-free and overall survival is the focus of subsequent studies to follow this pilot trial.

4.0 VACCINE PREPARATION

4.1 GM2 is provided by Progenics. GLOBO-H, Lewis-Y, TF(c), Tn (c), and sTn (c) are synthesized in the laboratory of Dr. Sam Danishefsky at the center. MUC-1 is produced at the core facility at MSKCC. For glycosylation, the MUC-1 was shipped to the University of Copenhagen, Glycobiology Group. The glycosylation was carried out by GalNAc transferase using UDP-N-GalNAc as substrate. The product was shipped back to MSKCC after purification by reverse phase HPLC.

4.2 QS-21 is obtained from Aquila Biopharmaceuticals in 100 mg vials as a white powder and is stored at −30 degrees Celsius. This is suspended initially in PBS as it is less soluble in normal saline and then final dilutions are made in normal saline. QS-21 is passed through a 0.22 micrometer filter immediately prior to use.

4.3 Conjugation to KLH is accomplished with three different conjugation procedures: direct amination (ozonolysis) for GM2, the M2C2H bifunctional linker group for Globo H and Le Y, and the MBS bifunctional linker group for the four mucin antigens.

4.4 The sterility of the conjugate is confirmed by passage through a 0.22 micrometer filter and it is stored in frozen normal saline at −30 to −80 degrees Celsius.

4.5 Vials are released for use following standard lot release testing (approximately five weeks).

5.0 TREATMENT SCHEDULE AND DOSE
5.1 Vaccine Contains:

[GM2(10 mcg)/TF(c)(3 mcg)/sTn(c) (3 mcg)/Globo-H (10 mcg)/MUC1-1-G5(3 mcg)/Le^Y(10 mcg)/Tn(c)(3 mcg)]-KLH (≈400 mcg) with adjuvant QS21(100 mcg)

5.2 Immunization Schedule

The vaccine will be administered at weekly intervals for 3 doses. This will be followed by a four week break and then a fourth vaccination. There will then be an eight week break and then a fifth vaccination, followed by additional immunizations every twelve weeks for 24 months total (as long as patient remains on study).

IMMUNIZATION SCHEDULE

WEEK #
1
2
3
7
15

VACCINE #
1
2
3
4
5

5.3 Dose Administration and Modification

5.3.1 No dose escalation or dose modification will be performed. Systemic toxicity has not been seen with the previous vaccine studies. Systemic toxicity >grade II (with the exception of fever without infection) thought related to vaccination would result in removal of the patient from study and suspension of the protocol pending investigation.

5.3.2 The preparation will be administered subcutaneously to a site in the shoulders, buttocks, or thighs. It will be administered in one syringe, and will be supplied in approximately 1 cc total volume.

6.0 EVALUATION DURING STUDY
6.1 Immune Function (Summarized in Table)
6.1.1 Antibody Response:

Peripheral blood (20-30 ml) will be drawn according to the schedule in table 8.3 with the exception of week 0, 7, and 9 at which time 50-60 ml will be collected for antibody testing. Thereafter, blood will be drawn at 12-week intervals as the patients return for booster immunizations. Antibodies against various antigens will be studies by ELISA, and against human tumor cell lines by FACS when appropriate.

6.2 Clinical and Laboratory Assessment:
6.2.1 Clinical and Laboratory Assessment Schedule:

The clinical and laboratory assessment schedule is outlined in Section 8.3 and includes parameters to assess the safety of the vaccine, as well as evaluate for signs of disease recurrence and progression. Abnormal findings will be evaluated per standard medical practice, and the abnormality will be classified as related to treatment, disease progression, or neither.

6.2.3 Extent of Disease Evaluation:

All patients are by definition without clinical or radiographic evidence of disease at protocol entry.

6.2.4 Radiographic Imaging

(CT abdomen and pelvis) will be obtained q 6 months while on study, or if any clinical symptoms/examination findings warrant further evaluation, or if serum CA-125 rises to ≧70 (per time to treatment failure criteria), confirmed by repeat value; or at any time at the discretion of the investigator.

6.2.5 Length of Follow-Up:

The primary endpoint of the study in this pilot trial is safety. Patients will be followed for the duration of the study, but based on previous trials, antibodies are generally present by the seventh week, and we will proceed with the proposal for additional studies to evaluate efficacy if no systemic toxicity is seen in any patient at the ninth week assessment. An additional 8-12 weeks would be required for processing before patients could be enrolled on the polyvalent study, allowing ample time for follow-up of the pilot trial. Patients will be followed until time to treatment failure, or until all vaccinations are completed (maximum 24 months).

6.3 Summary of Evaluation:

SUMMARY OF CLINICAL, LABORATORY, AND

IMMUNE ASSESSMENTS

week #

0^a
1
2
3
5
7
9
13
15
17
27^c

vaccine #

1
2
3

4

5

V

Office Visit
*
*
*
*
*
*
*
*
*
*
*

Hx and PE
*

*
*

*
*
*
*
*
*

CA-125
*

*

*
*
*

*

CBC, diff
*

*
*
*
*
*
*
*
*
*

Hepatic profile +
*

*
*
*
*
*
*
*
*
*

creatinine

Amylase
*

*
*
*
*
*
*
*
*
*

Urinalysis
*

*

*

*

*

PT
*

Stool guaiac^b
*

*

*

*

TSH
*

*

Immune^d

*

*
*
*
*
*
*

bloods

^a= pretreatment evaluation, within 3 weeks

^b= stool guaiac may be obtained by digital exam or cards collected by patient

^c= following week 27, visits + laboratory studies + immunization q 3 months, CT scan q 6 months while on study

^d= immune bloods routinely consist of 20-30 ml collected in 3 red top tubes. In order to obtain sufficient serum to evaluate for multiple antibodies, 6 tubes will be collected instead of 3 at the pre-vaccination visit; and at week 7 and 9 only.

7.0 BIOSTATISTICAL CONSIDERATIONS
Endpoints:

The primary endpoints of this pilot trial are safety and confirmation of immunogenicity in the polyvalent setting. No systemic toxicity has occurred with the administration of monovalent vaccines at the center. Toxicity is not expected with this preparation. Following this pilot, additional studies with efficacy as the endpoint will be proposed. This pilot trial would be suspended pending investigation for any systemic toxicity thought related to vaccine in any patient. The same criteria for immunogenicity will be used as that of the individual pilot trials: patients must have IgM titer >1:80, or a four fold increase in prevailing antibody titer if present at baseline. Nine patients will be accrued, and >5 of 9 patients should meet these criteria for three or more antigens in order to proceed with this construct in additional studies. In prior trials, antibodies are generally present by completion of the fourth vaccination (week 7). If no systemic toxicity is seen by the week 9 assessment in these patients, we will proceed with proposals for phase II studies with efficacy endpoints.

While not the endpoint of this pilot, patients would be removed from study for relapse as defined below. Time to treatment failure will be simply defined based on data from Rustin et al.⁴²Treatment failure can be characterized by 1) physical examination evidence of disease recurrence, radiographic evidence of disease recurrence (biopsy will be performed at the discretion of the principal investigator but is not required); or 3) CA-125 elevation to twice the upper limits of normal (ie. ≧70), confirmed by a second sample also ≧70 U/ml. Time to treatment failure for biochemical relapse is recorded as the date of the first sample ≧70 U/ml.

The secondary endpoint of this pilot trial is to characterize the nature and duration of the immune response. Peripheral blood (20-30 ml) will be drawn as indicated in the table. Antibodies against the individual antigens will be studies by ELISA, and against the appropriate human tumor antigen FACS using human tumor cell lines expressing the respective antigen.

REFERENCES

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2. Barnhill D R, Hoskins W J, Heller P B, et al: The second look surgical reassessment for epithelial ovarian cancer. Gynecologic Oncology 19:148-, 1984

3. Cain J M, Saigo P E, Pierce V R, et al: A review of second look laparotomy for ovarian cancer. Gynecologic Oncology 23:14-, 1986

4. Rubin S C, W. J. H, Saigo P E, et al: Recurrence following negative second look laparotomy for ovarian cancer. American Journal of Obstetrics and Gynecology 159:1094-, 1988

5. Livingston P O, Zhang S, Lloyd K O: Carbohydrate vaccines that induce antibodies against cancer. Part I. Rational. Immunol Immunother 45:1-9, 1997

6. Jones P C, Sze L L, Liu P Y, et al: Prolonged survival for melanoma patients with elevated IgM antibody to oncofetal antigen. Journal of the National Cancer Institute 66:249-54, 1981

7. Zhang H, Zhang S, Cheung N K, et al: Antibodies can eradicate cancer micrometastasis. Cancer Research 58:2844-99, 1998

8. Livingston P O, Wong G Y C, Alduri S, et al: Improved survival in AJCC stage III melanoma patients with GM2 antibodies: a randomized trial of vaccination with GM2 ganglioside. Journal of Clinical Oncology 12:1036-44, 1994

9. Reithmuller G, Schneider-Gadicke E, Schlimok G, et al: Randomized trial of monoclonal antibody for adjuvant therapy of resected Dukes C colorectal carcinoma. Lancet 343:1177-1183, 1994

10. Livingston PO: The cases for melanoma vaccines that induce antibodies., in Kirkwood J M (ed): Molecular Diagnosis Prevention and Treatment of Melanoma, Marcel Dekker, Inc., 1997

11. Zhang S, Helling F, Lloyd KO, et al: Increased tumor cell reactivity and complement dependent cytotoxicity with mixtures of monoclonal antibodies against different gangliosides. Cancer Immunology and Immunotherapy 40:88-94, 1995

12. Feizi T: Demonstration by monoclonal antibodies that carbohydrate structures of glycoproteins and glycolipids are onco-developmental antigens. Nature 314:53-57, 1985

13. Fung P Y S, Madej M, Koganty R R, et al: Active specific immunotherapy of a murine mammary adenocarcinoma using a synthetic tumor associated glycoconjugate. Cancer Research 50:4308-4314, 1990

14. Singhal A, Fohn M, Hakomori S I: Induction of a-N-acetylgalactosamine-O-serine/threonine(Tn) antigen mediated cellular immune response for active immunotherapy in mice. Cancer Research 51:1406-1411, 1991

15. Zhao X J, Cheung N K: GD2 Oligosaccharide: target for cytotoxic T lymphocytes. Journal of Experimental Medicine 182:67-74, 1995

16. Livingston P O: Augmenting the immunogenicity of carbohydrate antigens. Seminars in Cancer Biology 6:357-366, 1995

17. Ghossein R, Scher H, Gerald W, et al: Detection of circulating tumor cells in patients with localized and metastatic prostate cancer. Journal of Clinical Oncology 13:1195-1200, 1995

18. Livingston P O, Natoli J, Jones Calves M, et al: Vaccines containing purified GM2 ganglioside elicit GM2 antibodies in melanoma patients. Proceedings of the Natl Acad Sci USA 84:2911-2915, 1987

19. MacLean G D, Bowen-Yachyn M B, Samuel J, et al: Active immunization of human ovarian cancer patients against a common carcinoma (Thomsen-Friedenreich) determinant using a synthetic carbohydrate antigen. Journal of Immunotherapy 11:292-305, 1992

20. Adluri S, Helling F, Calves M J, et al: Immunogenicity of synthetic TF and sTn-KLH conjugate in colorectal carcinoma patients. Cancer Immunology and Immunotherapy 41:185-192, 1995

21. Nakada H, Inoue M, Numata Y, et al: Epitopic structure of Tn glycophorin A for an anti-Tn antibody (MLS128). Proceedings of the Natl Acad Sci USA 90:2495-2499, 1993

22. Zhang S, Walberg L A, Ogata S, et al: Immune sera and monoclonal antibodies define two configurations for the sialyl Tn tumor antigen. Cancer Research 55:3364-3368, 1995

23. Bilodeau M T, Park T K, Hu S T, J. T./, et al: Total synthesis of a human breast tumor associated antigen. Journal of the American Chemical Society 117:7840-7841, 1995

24. Ragupathi G, Slovin S, Adluri S, et al: A fully synthetic globo-H carbohydrate vaccine induces a focused humoral response in prostate cancer patients: a proof of principle. Angewandte Chemie 38:563-566, 1999

25. Kudryashov V, Kim H M, Ragupathi G, et al: Immunogenicity of synthetic conjugates of Lewis-Y oligosaccharide with protein in mice: towards the design of anticancer vaccines. Cancer Immunology and Immunotherapy 45:281, 1998

26. Slovin S F, Ragupathi G, Adluri S, et al: Immunogenicity of a fully synthetic globo-H hexasaccharide conjugate in man. Proc Natl Acad Sci USA 96:5710-5715, 1999

27. Sabbatini P, Kudryashov V, Ragupathi G, et al: Immunization of ovarian cancer patients with a synthetic Lewis-Y protein conjugate vaccine: a phase I trial. Intl J Cancer 87 (1): 79-85, 2000.

28. Zhang S, Walberg L A, Helling F, et al: Augmenting the immunogenicity of synthetic MUC-1 vaccines in mice. Cancer Research 55:3364-3368, 1996

29. Gilewski T, Adluri S, Zhang S, et al: Vaccination of high-risk breast cancer patients with Mucin-1 keyhole limpet hemocyanin conjugate plus QS-21. Clinical Cancer Research 6(5):1693-701, 2000.

30. Adluri S, Gilewski T, Zhang S, et al: Specificity analysis of sera from breast cancer patients vaccinated with Muc-1-KLH plus QS-21. British Journal of Cancer 79:1806-1812, 1999

31. Ragupathi G, Park T K, Zhang S, et al: Immunization of mice with the synthetic hexasaccharide Globo H results in antibodies against human cancer cells. Angewandte Chem Int Engl:125-128, 1997

32. Livingston P O: Approaches to augmenting the immunogenicity of melanoma gangliosides: from whole melanoma cells to ganglioside-KLH conjugate vaccines. Immunological Reviews 145:147-166, 1995

33. Chapman P B, Morissey D M, Pangeas K S, et al: Induction of antibodies against GM2 ganglioside by immunizing melanoma patients using GM2-KLH+ QS21 vaccine: a dose response study. Clinical Cancer Research in press, 1999

34. Helling F, Shang Y, Calves M, et al: Increased immunogenicity of GD3 conjugate vaccines: comparison of various carrier proteins and selection of GD3-KLH for further testing. Cancer Research:197-203, 1994

35. Kensil C R, Patel U, Lennick M: Separation and characterization of saponins with adjuvant activity from Quillaja saponin Molina cortex. Journal of Immunology 146:431-436, 1991

36. Kim S K, Ragupathi G, Musselli C, et al: Comparison of the effect of different immunological adjuvants on the antibody and T-cell response to immunization with MUC1-KLH and GD3-KLH conjugate carrier vaccines. Vaccine 18:597-603, 2000

37. Marciani D J, Kensil C R, Beltz G A: Genetically engineered subunit vaccine against FeLV: protective immune response in cats. Vaccine 9:89-96, 1991

38. Livingston P O, Adluri S, Helling F, et al: Phase I trial of immunological adjuvant QS-21 with a GM2 ganglioside-keyhole limpet hemocyanin conjugate vaccine in patients with malignant melanoma. Vaccine 12:1275-1280, 1994

39. Zhang S, Zhang H, Cordon-Cardo C, Reuter V, et al. Selection of tumor antigens as targets for immune attack using immunohistochemistry: II. Blood Group-Related Antigens. Int J Cancer 73: 50-56, 1997.

40. Zheng S, Cordon-Cardo C, Zhang H, Reuter V, et al. Selection of tumor antigens as targets for immune attack using immunohistochemistry: I. Focus on gangliosides. Int J Cancer 73: 42-49, 1997.

41. Zheng S, Zhang HHHS, Cordon-Cardo C, Ragupathi G, et al. Selection of tumor antigens for immune attack using immunohistochemistry: Protein antigens. Clin Cancer Res 4: 2669-2676, 1998.

42. Rustin G J, Nelstrop A E, Bentzen S M, et al: Use of tumour markers in monitoring the course of ovarian cancer. Ann Oncol 10:21-7, 1999

Example 2
Heptavalent Vaccine Immunogenicity Trial 1N Mice
Methods
Serological Analyses
1. ELISA (Enzyme-Linked Immunosorbent Assay):

2. Cell Surface Reactivity Determined by FACS:

The cell surface reactivity of immune sera was tested on human MCF-7 and LSC cell lines. Single cell suspensions of 2×10⁵cells/tube were washed in PBS with 3% fetal calf serum (FCS) and 0.01M NaN₃and incubated with 20 μl of 1:20 diluted sera or monoclonal antibody mAb for 30 min on ice. After two washes with 3% FCS in PBS, 20 μl of 1:15 diluted goat anti-mouse IgM or IgG-labeled with fluorescein-isothiocyanate (FITC, Southern Biotechnology Associates Inc. Birmingham, Ala.) was added, and the mixture incubated for 30 min. After a final wash, the positive population and mean fluorescence intensity of stained cells were differentiated using FACScan, Becton & Dickinson Immunocytometry, San Jose, Calif.

Immunizaton of mice with Heptavalent-KLH Conjugates plus

ELISA
GPI100 Or QS21.

ELISA plate
mice immunized with . . ./
pre vacc.
post vacc.
Mar. 19, 2001

coated with . . .
(Group#)
(IgG/IgM)
(IgG/IgM)
Comments

GM2
GM2 (group #1)
0/0
0/0

GloboH (group#2)

0/0

LeY (group #3)

0/0

Muc1-G5 (group #4)

0/0

STn(c) (group #5)

0/0

TF(c) (group #6)

0/0

Tn(c) (group #7)

0/0

Globo H
GM2 (group #1)

GloboH (group#2)
0/0
640/5120

LeY (group #3)

Muc1-G5 (group #4)

STn(c) (group #5)

TF(c) (group #6)

Tn(c) (group #7)

LeY
GM2 (group #1)

0/0

GloboH (group#2)

0/0

LeY (group #3)
0/0
640/2560

Muc1-G5 (group #4)

0/0

STn(c) (group #5)

0/160

TF(c) (group #6)

0/40

Tn(c) (group #7)

0/40

Muc1-G5
GM2 (group #1)

0/320

GloboH (group#2)

0/160

LeY (group #3)

0/160

Muc1-G5 (group #4)
0/0
2560+/1280

STn(c) (group #5)

40/80

TF(c) (group #6)

40/80

Tn(c) (group #7)

0/320

mAb.
C595

2560/

B55

/<5120+++

STn(c)
GM2 (group #1)

0/0

GloboH (group#2)

0/0

LeY (group #3)

0/0

Muc1-G5 (group #4)

0/0

STn(c) (group #5)
0/0
5120/320

TF(c) (group #6)

0/0

Tn(c) (group #7)

0/0

mAb.
cc49

1280/0

Tf(c)
GM2 (group #1)

0/40

GloboH (group#2)

40/80

LeY (group #3)

40/40

Muc1-G5 (group #4)

5120+/160

STn(c) (group #5)

5120+/320

TF(c) (group #6)
0/0
5120+/320

Tn(c) (group #7)

5120+/640

mAb.
JAA-F11

0/

A78-6/A7

/640

Tn(c)
GM2 (group #1)

0/0

GloboH (group#2)

0/0

LeY (group #3)

0/0

Muc1-G5 (group #4)

5120+/160

STn(c) (group #5)

5120+/320

TF(c) (group #6)

5120+/320

Tn(c) (group #7)
0/0
5120+/2560

mAb.
5F4

/5120++

HB-Tn1

/5120

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

8.
Heptavalent-KLH +
Tn(c)
1
0/0
5120+/160

100 ug GPI-100

2
0/0
5120/160

(200 ul/mouse)

3
0/0
5120/160

4
0/0
5120++/640

5
0/40
5120+/320

Tf(c)
1
0/0
5120/160

2
0/0
5120/160

3
0/0
5120/160

4
0/0
5120+/320

5
0/40
5120+/640

sTN(c)
1
0/0
5120/640

2
0/0
1280/640

3
0/0
5120/640

4
0/0
5120/320

5
0/0
1280/320

MUC1-1G5
1
0/0
5120+/0

2
0/0
5120+/80

3
0/0
5120+++/160

4
0/0
5120++/40

5
0/0
5120+++/80

Ley
1
0/0
0/40

2
0/0
320/640

3
0/0
0/160

4
0/0
80/40

5
0/0
0/640

Globo H
1
0/80
40/640

2
0/80
0/640

3
0/80
0/640

4
0/160
40/1280

5
0/160
0/2560

GM2
1
0/0
0/40

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

Apr. 2, 2001

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

9.
Heptavalent-KLH +
Tn(c)
1
0/0
640/40

100 ug GPI-100

2
0/0
640/0

(Batch J)

3
0/0
5120/40

(200 ul/mouse)

4
0/0
5120+/0

5
0/0
1280/40

Tf(c)
1
0/0
1280/80

2
0/0
1280/40

3
0/0
5120+/40

4
0/0
5120++/40

5
0/0
2560/40

sTN(c)
1
0/0
320/80

2
0/0
320/160

3
0/0
640/160

4
0/0
640/80

5
0/0
80/320

MUC1-1G5
1
0/0
2560/0

2
0/0
640/0

3
0/0
640/0

4
0/0
640/0

5
0/0
2560/80

Ley
1
0/0
0/0

2
0/0
0/80

3
0/0
0/0

4
0/0
0/0

5
0/0
160/1280

Globo H
1
0/80
0/160

2
0/80
0/320

3
0/80
0/160

4
0/80
0/320

5
0/80
40/320

GM2
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

Apr. 2, 2001

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

10.
Heptavalent-KLH +
Tn(c)
1
0/0
5120++/320

100 ug GPI-100 +

2
0/0
5120/320

polysorbate 80

3
0/40
5120+/1280

(200 ul/mouse)

4
0/0
5120+/640

5
0/0
2560/320

Tf(c)
1
0/0
5120+/320

2
0/0
5120+/160

3
0/0
5120+/640

4
0/0
5120+/640

5
0/0
5120+/320

sTN(c)
1
0/0
320/640

2
0/0
320/1280

3
0/0
1280/1280

4
0/0
640/40

5
0/0
320/320

MUC1-1G5
1
0/0
1280/40

2
0/0
5120/80

3
0/0
5120/160

4
0/0
2560/160

5
0/0
5120/40

Ley
1
0/0
0//0

2
0/0
0/0

3
0/0
0/640

4
0/0
0/640

5
0/0
0/80

Globo H
1
0/40
80/640

2
0/80
40/2560

3
0/320
0/2560

4
0/160
0/2560

5
0/80
0/640

GM2
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

Apr. 2, 2001

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

11.
Heptavalent-KLH+ +
Tn(c)
1
0/0
5120/160

10 ug QS-21

2
0/0
5120+/160

(200 ul/mouse)

3
0/40
5120+++/160

4
0/80
2560/320

5
0/0
5120+/80

Tf(c)
1
0/40
5120+/320

2
0/0
5120++/640

3
0/160
5120++640

4
0/320
2560/640

5
0/40
5120++/320

sTN(c)
1
0/0
40/40

2
0/0
2560/640

3
0/0
5120/160

4
0/0
1280/80

5
0/0
5120/640

MUC1-1G5
1
0/0
1280/160

2
0/0
2560/80

3
0/0
5120/80

4
0/0
2560/320

5
0/0
5120++/80

Ley
1
0/0
0//0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
40/40

Globo H
1
0/80
40/320

2
0/80
80/320

3
0/80
40/640

4
40/160
0/640

5
0/320
0/2560

GM2
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

Apr. 16, 2001

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

12.
Heptavalent-KLH +
Tn(c)
1
0/40
2560/160

3 ug ER-803022

2
0/0
640/160

(200 ul/mouse)

3
0/40
320/320

4
0/0
160/160

5
0/0
2560/160

Tf(c)
1
0/0
2560/40

2
0/0
2560/40

3
0/0
640/160

4
0/0
320/80

5
0/0
2560/0

sTN(c)
1
0/0
0/40

2
0/0
40/80

3
40/40
80/160

4
0/0
160/160

5
0/0
40/0

MUC1-1G5
1
0/0
80/0

2
0/0
80/0

3
0/0
80/40

4
0/0
40/80

5
0/0
40/0

Ley
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/80

5
0/0
0/0

Globo H
1
0/80
0/320

2
0/160
40/1280

3
0/320
0/320

4
80/160
160/1280

5
40/160
320/640

GM2
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

Apr. 16, 2001

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

13.
Heptavalent-KLH +
Tn(c)
1
0/40
40/320

10 ug ER-803732

2
0/0
40/40

(200 ul/mouse)

3
0/0
320/160

4
0/40
160/160

5
0/40
160/80

Tf(c)
1
0/0
160/160

2
0/0
320/40

3
0/40
640/160

4
0/40
320/160

5
0/0
320/160

sTN(c)
1
0/0
40/80

2
0/0
0/80

3
0/0
0/320

4
0/160
40/320

5
0/40
40/160

MUC1-1G5
1
0/0
640/40

2
0/0
0/40

3
0/0
40/80

4
0/40
80/160

5
0/0
160/80

Ley
1
0/0
0/0

2
0/0
0/0

3
0/40
40/320

4
0/0
0/40

5
0/0
0/80

Globo H
1
40/80
80/160

2
0/160
40/320

3
0/40
80/320

4
0/80
0/160

5
80/160
160/320

GM2
1
0/0
0/0

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug),

Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Polysorbate 80, 4 mg/ml in final vaccine.

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21.

ELISA (IgG/IgM)
FACS (IgG/IgM)

Group #
Antigen
Mice #
Pre-vacc.
Post-vacc
Pre-vacc.
Post-vacc.
Comments

14.
30 ug KLH +
Tn(c)
1
0/0
0/160

100 ug GPI-100

2
0/0
0/40

(100 ul/mouse)

3
0/0
0/0

4
0/0
0/160

5
0/40
0/640

Tf(c)
1
0/40
0/320

2
0/40
0/160

3
0/0
0/80

4
0/0
0/320

5
0/160
40/640

sTN(c)
1
0/0
0/80

2
0/0
0/40

3
0/0
0/0

4
0/0
0/320

5
0/0
0/80

MUC1-1G5
1
40/40
0/160

2
0/40
0/80

3
0/0
0/80

4
0/0
0/320

5
0/0
0/320

Ley
1
0/0
0/40

2
0/0
0/0

3
0/0
0/0

4
0/0
0/0

5
0/0
0/0

Globo H
1
0/320
40/1280

2
0/320
0/640

3
0/80
0/1280

4
0/160
0/640

5
0/160
40/640

GM2
1
0/0
0/160

2
0/0
0/40

3
0/0
0/0

4
0/0
0/320

5
0/0
0/160

KLH
1
0/0
5120++/320

2
0/40
5120++/160

3
0/0
5120++/320

4
0/0
5120++/640

5
0/40
5120++/320

Immunization of mice with Heptavalent-KLH C njugates* plus GPI-100 r QS-21.

FACS
% positive cells

Group #
MCF-7 (IgG/IgM)
LSC (IgG/IgM)

(mice immunized with . . . )
Mice #
Pre-vacc.
Post-vacc.
1:200 dilut.
Pre-vacc.
Post-vacc.
1:200 dilut.

1. 3 ug GM2-KLH +
1
11.79/10.68
21.45/11.79
15.73/0.38
10.90/9.58
6.91/2.93
6.56/0.14

100 ug GPI-100
2
10.23/10.69
4.80/1.49
2.34/0.0
10.90/10.45
5.99/3.45
1.45/0.59

(100 ul/mice)
3
9.50/10.74
6.95/15.79
0.99/0.21
11.29/11.11
7.79/1.53
6.41/0.23

4
9.81/9.68
3.41/12.63
0.99/2.06
9.76/11.06
6.94/1.75
3.42/0.02

5
10.81/10.42
10.43/3.15
12.29/0.11
10.13/10.76
4.40/1.67
0.40/0.10

2. 3 ug GloboH-KLH +
1
10.63/9.93
5.79/17.26
6.60/0.19
9.87/10.99
7.08/2.77
9.55/0.25

100 ug GPI100
2
10.08/10.67
16.60/27.63
10.54/6.75
10.0/10.41
8.9/3.43
1.29/0.52

(100 ul/mice)
3
11.03/10.09
27.21/40.86
27.58/2.30
10.42/10.61
11.56/1.15
7.60/0.02

4
10.16/11.36
1.92/13.77
2.30/1.03
10.57/11.04
5.29/2.43
3.81/0.24

5
11.94/10.82
24.61/12.97
20.32/3.62
10.79/10.72
10.58/2.54
1.25/0.20

3. 3 ug Ley-KLH +
1
11.01/9.97
85.01/43.57
41.26/1.73
10.22/10.10
89.17/44.27
13.40/1.87

100 ug GPI-100
2
9.95/9.69
47.75/78.17
4.86/3.43
10.49/8.39
91.69/79.9
7.64/7.04

(100 ul/mice)
3
10.41/10.58
69.55/10.95
20.53/0.12
11.30/9.47
95.57/21.25
24.67/0.16

4
11.93/10.03
91.08/0.76
21.29/0.0
10.96/9.60
81.5/6.24
9.08/0.38

5
12.46/11.18
42.94/36.67
13.66/1.87
10.98/10.61
12.74/52.16
1.05/1.87

4. 3 ug Muc-1G-5-KLH +
1
11.33/10.94
98.12/9.52
97.98/0.93
9.50/9.89
4.83/1.10
2.29/0.18

100 ug GPI-100
2
10.90/9.44
88.05/1.47
66.29/0.07
11.39/9.63
8.47/0.15
4.85/0

(100 ul/mice)
3
10.59/10.81
93.34/0.93
83.12/0.09
10.42/9.85
7.42/1.16
3.15/0.02

4
10.47/9.70
94.57/21.92
85.52/0.47
9.70/11.11
10.99/7.79
3.47/0.71

5
12.29/10.03
99.77/6.12
99.79/0.77
*11.05/10.49
63.71/1.82
28.90/0.71

5. 3 ug STn(c)-KLH +
1
9.56/9.77
13.95/1.74
1.29/0.13
10.10/10.73
95.14/4.42
86.94/0.50

100 ug GPI-100
2
9.91/10.59
15.95/1.79
12.70/0.23
10.20/11.18
98.65/19.42
88.58/0.59

(100 ul/mice)
3
10.72/10.55
6.88/2.81
6.23/0.02
11.31/11.46
97.78/31.98
95.31/0.36

4
9.62/9.52
4.62/1.69
3.18/0.14
10.11/9.78
94.14/1.19
86.65/0.09

5
10.77/10.71
17.96/2.16
7.17/0.3
10.71/0.05
97.66/7.28
87.09/0.38

6. 3 ug Tf(c)-KLH +
1
10.84/10.39
13.89/5.73
5.86/0.23
9.64/10.31
7.66/4.74
3.85/0.24

100 ug GPI-100
2
9.22/11.34
31.03/4.44
31.75/0.10
9.65/10.15
9.01/1.17
3.98/0.18

(100 ul/mice)
3
10.59/10.11
4.05/1.05
0.73/0.02
10.12/9.92
4.97/2.77
0.90/0.04

4
10.26/10.63
6.72/7.10
2.19/0.19
9.72/10.79
3.85/3.58
2.25/0.16

5
12.0/10.90
9.11/6.28
5.18/0.18
*11.54/10.09
11.71/5.0
12.76/0.64

7. 3 ug Tn(c)-KLH +
1
9.60/10.44
3.64/8.41
0.62/0.37
10.65/10.46
9.91/5.07
3.02/0.32

100 ug GPI-100
2
10.54/10.46
12.94/3.24
20.35/0.17
11.50/10.85
4.81/0.48
5.33/0.05

(100 ul/mice)
3
10.51/10.46
4.72/23.22
0.16/1.22
10.70/9.68
2.37/1.33
0.04/0.02

4
10.97/9.48
8.50/17.77
4.52/0.16
10.94/10.97
18.50/1.81
4.18/0.12

5
10.79/10.72
46.27/32.77
9.46/2.04
11.40/10.16
25.42/16.84
16.5/22.80

*DU145

+ control
IE-3
91.67, 95.15
+control
IE-3
95.73%

MLS128
77.07%

HMFG1
38.34%

MLS132
19.92, 4.52

49H8
84.90%

8. Heptavalent-KLH +
1
10.84/11.21
89.44/17.63
69.48/0.47
10.29/10.63
97.79/49.78
90.80/0.46

100 ug GPI-100
2
9.55/9.54
96.98/25.87
83.67/1.12
9.97/10.58
95.44/74.27
83.11/0.35

(200 ul/mice)
3
9.94/10.88
96.53/32.44
88.36/0.79
10.56/10.91
95.39/40.29
85.79/0.49

4
10.90/10.72
99.47/5.72
96.61/0.45
10.69/10.42
97.65/16.44
88.77/0.28

5
10.37/10.17
75.64/10.67
63.57/0.11
10.58/10.14
93.93/15.49
71.06/1.36

9. Heptavalent-KLH +
1
10.65/10.57
74.25/12.81
69.56/1.07
10.93/10.21
99.45/8.83
85.59/0.38

100 ug GPI-100
2
10.20/10.97
98.22/16.51
81.61/0.91
10.86/10.78
96.70/22.94
66.20/0.50

(batch J)
3
9.96/9.68
89.36/1.03
60.88/0.22
9.79/9.80
95.10/0.43
53.45/0.03

(200 ul/mice)
4
10.77/10.75
82.25/8.95
27.80/0.09
10.58/10.28
92.21/1.17
65.13/0.18

5
10.95/10.77
77.49/10.19
62.39/0.13

10. Heptavalent-KLH +
1
10.99/10.32
84.54/8.61
39.91/0.49
10.63/10.92
93.11/38.33
63.61/1.57

100 ug GPI-100 +
2
10.09/10.92
97.83/11.79
94.21/0.16
10.72/10.68
97.64/12.52
77.95/0.05

polysorbate 80
3
11.32/10.32
97.74/15.67
89.24/0.30
9.53/10.16
89.84/2.13
63.96/0.19

(200 ul/mice)
4
9.76/10.59
92.51/15.57
82.83/0.10
11.50/10.03
60.13/14.56
8.56/1.59

5
10.33/10.05
80.12/11.34
70.98/0.30

11. Heptavalent-KLH +
1
10.96/10.08
91.06/1.64
55.98/0.02
9.76/10.81
26.58/2.13
5.42/0.16

10 ug QS-21
2
9.88/10.41
94.84/2.32
72.07/0.02
9.80/11.58
88.16/22.37
34.36/0.94

(200 ul/mice)
3
11.0/10.57
99.34/9.99
93.96/0.84
9.86/10.79
87.20/11.70
76.90/0.14

4
11.05/10.65
88.58/3.78
61.69/0.13
10.07/10.45
71.56/3.79
26.42/0.15

5
10.86/10.27
81.44/6.27
69.68/0.14

12. Heptavalent-KLH +
1
18.54/11.29
67.73/1.59
26.33/0.18
10.98/9.97
16.98/1.97
6.40/0.09

3 ug ER803022
2
9.69/9.60
74.76/0.72
33.45/0.08
10.62/10.33
36.76/2.05
3.73/0.07

(200 ul/mice)
3
9.65/10.62
91.62/2.89
46.96/0.31
10.16/10.03
28.33/4.88
3.26/0.10

4
10.78/10.0
22.58/4.14
9.51/0.36

5
10.90/10.94
48.15/7.29
10.64/0.23

13. Heptavalent-KLH +
1
10.08/10.56
74.85/8.71
40.57/0.24
10.96/10.20
64.39/3.85
7.58/0.17

10 ug ER803732
2
11.03/10.91
36.35/5.07
4.79/0.07
9.84/10.19
3.67/11.73
0.47//0.73

(200 ul/mice)
3
10.22/10.54
65.94/30.22
7.87/0.63
10.83/10.07
66.06/25.19
8.66/0.82

4
10.75/10.07
91.69/12.15
22.96/0.41

5
10.87/11.04
35.45/6.88
1.38/0.11

14. 30 ug KLH +
1
9.42/11.35
13.72/9.84
10.08/2.29
10.85/10.49
5.49/4.48
3.29/2.53

100 ug GPI-100
2
12.14/11.31
17.50/2.09
6.41/0.0
10.58/10.44
10.57/3.53
14.38/0.21

(200 ul/mice)
3
9.82/10.97
1.64/1.05
0.13/0.02
9.19/11.45
15.10/1.03
11.63/0.01

4
11.20/11.84
13.25/2.14
10.05/0.12

5
10.51/9.95
8.98/5.40
1.38/0.06

Heptavalent: Tn(c) (3 ug), TF(c) (3 ug), sTn(c) (3 ug), MUC1-1G5 (3 ug), Ley (10 ug), Globo H (10 ug), and GM2 (10 ug).

New GPI-100 used for all groups except group 9 (batch J).

Third Series of Experiments
Polyvalent Conjugate Vaccine for Cancer

Tumor-specific antigens have been identified and pursued as targets for vaccines. The inventors' previous work has shown that monovalent vaccines utilizing the tumor antigens Globo H, Lewisy, GM2, glycosylated MUC-1, Tn(c), sTn(c), or TF(c) conjugated to KLH to be safe with local erythema and edema but minimal systemic toxicities. As a result of vaccination with these monovalent vaccines, most patients generated specific high titer IgM or IgG antibodies against the respective antigen-KLH conjugates. The present invention provides multivalent vaccines wherein the components of the monovalent vaccine are combined and administered with an adjuvant as treatment for cancer.

Vaccines consisting of a combination of tumor antigens administered with a saponin immunological adjuvant QS-21 or GPI-0100. The antigens are glycosylated MUC-1-G5, Globo H, GM2, Le^y, Tn(c), sTn(c), and TF(c). In each case the antigen is conjugated to Keyhole Limpet Hemocyanin (KLH).

The preferred ranges of the antigen and adjuvant doses are as follows:

- Glycosylated MUC-1-G5: 0.1 to 30 g;
- Globo H: 0.1 to 100 g;
- GM2: 0.1 to 100 g;
- Le^y: 0.1 to 60 g;
- Tn(c): 0.1 to 100 g;
- sTn(c): 0.1 to 100 g;
- TF(c): 0.1 to 30 g;
- QS-21: 25-200 g;
- GPI-0100: 1-25 mg.

Example 1
Comparison of the Immune Response after Immunization with Monovalent and Hexavalent-KLH Conjugate Vaccines Against Prostate Cancer

The immune response of the five initial patients receiving hexavalent vaccine with the immune responses of patients who had previously been immunized with the respective monovalent vaccines is compared in the following five tables. Shown are the reciprocal mean peak ELISA titer for IgM and IgG after immunization and FACS assay (% of positive cells/mean intensity) using the MCF-7 tumor cell line. The comparison for GM2-KLH is pending. Comparing the responses induced by monovalent and hexavalent vaccines, there was no significant difference in the antibody responses against any of the five antigens tested to date. Combination of six individual conjugates into a single vaccine does not significantly change the antibody response against the individual antigens.

Hexavalent Versus Monovalent: Prostate

Aug. 6, 2001

MCF-7

FACS

Patient
Elisa (TF-HSA)
IgM

Trial
Patient
Sera
IgM
IgG
%/Mean

protocol
M1
week 1
10
10
10/37

98-048

week 7
1280+
160
11/39

TF(c)-KLH +

week 9
1280
40
17/50

QS21
M2
week 1
10
0
10/21

dosage: 1 μg

week 7
1280++
10
52/54

week 9
1280+++
10
72/64

M3
week 1
0
0
11/135

week 7
1280++
160
2/28

week 9
1280++
1280
6/104

M4
week 1
0
0
10/32

week 7
160
10
18/43

week 9
160
160
26/47

M5
week 1
0
0
10/36

week 7
320
0
9/28

week 9
320
0
8/22

protocol
H1
week 1
20
0
11/64

00-064

week 7
1280
160
7/55

Hexavalent

week 12
1280
160
3/31

Conjgate +
H2
week 1
40
10
9/37

QS21

week 7
1280
160
21/50

TF(c)dosage:

week 12
640
160
17/43

3 μg
H3
week 1
40
0
10/35

week 7
1280
20
54/65

week 12
640
40
34/47

H4
week 1
80
0
10/26

week 7
1280
80
22/43

week 12
1280
20
19/54

H5
week 1
0
0
10/13

week 7
1280
320
57/26

week 12
1280
320
47/22

Controls
C1
Aug. 27, 1999
1280
1280

Hexavalent Versus Monovalent: Prostate

Aug. 10, 2001

MCF-7

Elisa

FACS

Patient
(Tn-HSA)

IgM

Trial
Patient
Sera
IgM
IgG
%/Mean

protocol 98-002
M1
week 1
0
80
10/22

Tn(c)-KLH + QS21

week 7
40
2560
7/18

dosage: 3 μg

week 9
80
2560
9/21

M2
week 1
10
80
11/26

week 7
320
5120
32/40

week 9
640
5120
37/42

M3
week 1
20
40
11/25

week 7
640
640
12/26

week 9
1280
1280
13/27

M4
week 1
40
40
10/49

week 7
640
1280
9/40

week 9
1280
1280
8/39

M5
week 1
10
80
11/25

week 7
1280
5120
12/26

week 9
1280
5120
13/27

protocol 00-064
H1
week 1
80
0
11/64

Hexavalent Conjgate +

week 7
320
1280
7/55

QS21

week 12
320
1280
3/31

Tn dosage: 3 μg
H2
week 1
320
10
9/37

week 7
1280
320
21/50

week 12
1280
320
17/43

H3
week 1
10
0
10/35

week 7
320
640
54/65

week 12
640
640
34/47

H4
week 1
40
160
10/26

week 7
640
5120
22/43

week 12
320
5120
19/54

H5
week 1
0
20
10/13

week 7
320
640
57/26

week 12
320
640
47/22

Controls
C2

1280+
640

Hexavalent Versus Monovalent: Prostate

Aug. 17, 2001

MCF-7

Elisa

FACS

Patient
(GloboH)

IgM

Trial
Patient
Sera
IgM
IgG
%/Mean

PROTOCOL 96-055
M1
week 1
0
0
11/40

GloboH - KLH +

week 7
20
0
9/30

QS21

week 9
20
0
9/40

dosage: 10 μg
M2
week 1
0
0
11/33

week 7
0
0
12/42

week 9
0
0
14/52

M3
week 1
20
0

week 7
640
0

week 9
640
0

M4
week 1
10
0
11/26

week 7
160
0
19/39

week 9
160
0
25/39

M5
week 1
40
0
10/26

week 7
160
0
17/38

week 9
off study
off study

PROTOCOL 00-064
H1
week 1
40
0
11/41

Hexavalent

week 7
160
0
9/36

Conjgate + QS21

week 12
160
80
6/27

GloboH dosage:
H2
week 1
160
0
11/33

10 μg

week 7
640
0
11/36

week 12
320
0
15/40

H3
week 1
40
0
11/29

week 7
20
0
56/59

week 12
20
0
43/46

H4
week 1
80
0
10/34

week 7
160
0
21/46

week 12
80
0
16/44

H5
week 1
40
0
10/15

week 7
80
0
64/35

week 12
80
0
45/27

Controls
C3
week 26

640

C4

1280

Hexavalent Versus Monovalent: Prostate

Aug. 31, 2001

MCF-7

Elisa

FACS

Patient
Ley-Cer

IgM

Trial
Patient
Sera
IgM
IgG
%/Mean

PROTOCOL 00-075
M1
week 1
0
0
11/23

LewY-MMCCH-KLH

week 7
0
0
13/26

dosage: 20 μg

week 9
0
0
24/92

M2
week 1
0
0
10/25

week 7
0
0
20/32

week 9
0
0
14/24

M3
week 1
0
0
11/30

week 7
40
80
8/20

week 9
20
40
14/41

M4
week 1
0
0
11/46

week 7
0
0
10/50

week 9
0
10
9/44

M5
week 1
0
0
10/50

week 7
40
0
3/30

week 9
0
10
18/63

PROTOCOL 00-064
H1
week 1
0
0
11/41

Hexavalent Conjgate +

week 7
0
0
9/36

QS21

week 12
0
0
6/27

Ley dosage: 10 μg
H2
week 1
0
0
11/33

week 7
0
0
11/36

week 12
0
0
15/40

H3
week 1
0
0
11/29

week 7
10
0
56/59

week 12
0
0
43/46

H4
week 1
0
10
10/34

week 7
10
10
21/46

week 12
10
0
16/44

H5
week 1
0
0
10/15

week 7
0
0
64/35

week 12
0
0
45/27

Controls
C5

2560

C6

640

Hexavalent Versus Monovalent: Prostate

Aug. 19, 2001

MCF-7

Elisa

FACS

Patient
(MUC33G5)

IgM

Trial
Patient
Sera
IgM
IgG
%/Mean

PROTOCOL 99-23
M1
week 1
0
0
10/25

MUC33G 5 Site -

week 7
160
640
17/31

KLH + QS21

week 9
160
640
31/45

dosage: 3 μg
M2
week 1
0
0
10/29

week 7
2560
640
38/53

week 9
2560
640
35/43

M3
week 1
0
20
10/28

week 7
2560
160
36/57

week 9
2560
320
43/60

M4
week 1
0
0
11/41

week 7
2560
80
12/35

week 9
640
320
12/38

M5
week 1
0
0
11/30

week 7
40
0
61/65

week 9
40
80
59/67

PROTOCOL 00-064
H1
week 1
0
0
11/41

Hexavalent

week 7
20
640
9/36

Conjgate + QS21

week 12
0
160
6/27

MUC33 dosage: 3 μg
H2
week 1
0
0
11/33

week 7
0
40
11/36

week 12
0
80
15/40

H3
week 1
0
0
11/29

week 7
160
160
56/59

week 12
40
320
43/46

H4
week 1
0
20
10/34

week 7
40
320
21/46

week 12
40
160
16/44

H5
week 1
0
0
10/15

week 7
40
160
64/35

week 12
0
80
45/27

Controls
C7

2560
640

Immunization of mice with Heptavalent-KLH Conjugates* plus GPI-100 or QS-21

Mean Value:

Nov. 30, 2001

LSC

ELISA
FACS
MCF-7
# LSC

Pre
Post
Pre
Post
1:200
Pre
Post
1:200
CDC(MCF-7)

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
Mice #
Pre
Post

1. 3 ug GM2-KLH +
Tn
0
0
0
0
10.43%
10.44%
9.40%
8.97%
6.47%
0.55%
10.59%
10.60%
6.41%
1.92%
3.63%
0.22%

100 ug GPI-100
Tf

(100 ul/mice)
sTn

Muc1-G5

Ley

globo H

GM2

2. 3 ug GloboH-
Tn
0
0
640
5120
10.77%
10.57%
15.22%
22.50%
13.47%
2.78%
10.33%
10.75%
7.08%
2.46%
4.70%
0.25%

KLH +
Tf

10.08%
10.57%
8.01%
32.59%
6.86%
7.39%

100 ug GPI100
sTn

(mice#1

(100 ul/mice)
Muc1-G5

re-

Ley

tested.)

globo H

GM2

3. 3 ug Ley-KLH +
Tn
0
0
640
2560
11.15%
10.34%
67.27%
34.02%
20.32%
1.43%
10.79%
9.63%
74.13%
40.76%
11.12%
2.26%
3-1
5.94%
46.42%

100 ug GPI-100
Tf

3-2
4.47%
75.05%

(100 ul/mice)
sTn

3-3
4.49%
9.21%

Muc1-G5

3-4
22.5%
119.0%

Ley

3-5
11.02%
61.7%

globo H

GM2

ELISA
FACS
MCF-7
LSC

Pre
Post
Pre
Post
1:200
Pre
Post
1:200
CDC(MCF-7)

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
Mice #
Pre

4. 3 ug Muc-1G-
Tn
0
0
2560+
1280
11.12%
10.12%
94.77%
7.99%
86.54%
0.46%
10.25%
10.12%
7.93%
2.55%
3.44%
0.23%
4-1
3.30%

5-KLH +
Tf

4-2
6.85%

100 ug GPI-100
sTn

4-3
14.0%

(100 ul/mice)
Muc1-

4-4
4.49%

G5

4-5
4.23%

Ley

globo H

GM2

5. 3 ug STn(c)-KLH +
Tn
0
0
5120
320
10.12%
10.23%
11.88%
2.04%
6.11%
0.16%
10.49%
8.64%
96.67%
12.86%
88.91%
0.38%
5-1
6.83%

100 ug GPI-100
Tf

5-2
10.91%

(100 ul/mice)
sTn

5-3
6.36%

Muc1-

5-4
7.11%

G5

5-5
4.37%

Ley

globo H

GM2

6. 3 ug Tf(c)-KLH +
Tn
0
0
5120
320
10.58%
10.67%
10.56%
4.92%
9.14%
0.14%
9.78%
10.29%
6.37%
3.06%
2.74%
0.16%

100 ug GPI-100
Tf

(100 ul/mice)
sTn

Muc1-

G5

Ley

globo H

GM2

7. 3 ug Tn(c)-KLH +
Tn
0
0
5120+
2560
10.48%
10.31%
15.21%
17.10%
7.02%
0.79%
11.04%
10.42%
12.20%
5.11%
5.81%
4.66%

100 ug GPI-100
Tf

(100 ul/mice)
sTn

Muc1-G5

Ley

globo H

GM2

KLH

LSC

ELISA
FACS
MCF-7
# LSC

Pre
Post
Pre
Post
1:200
Pre
Post
1:200
CDC(MCF-7)

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
Mice #
Pre
Post

8. Heptavalent-
Tn
0
10
5120+
320
10.32%
10.5%
91.61%
18.46%
80.34%
0.59%
10.43%
10.54%
96.04%
39.25%
83.91%
0.59%
8-1
0.75%
2.99%

KLH +
Tf
0
10
5120
320
10.63%
10.14%
98.92%
24.41%
85.27%
7.44%

8-2
1.0%
12.63%

100 ug GPI100
sTn
0
0
2560
640
(mice

8-3
−2.23%
44.48%

(200 ul/mice)
Muc1-G5
0
0
5120++
80
#1

8-4
−3.12%
24.77%

Ley
0
0
80
160
re-

8-5
7.65%
27.28%

globo H
0
80
10
1280
tested)

VK9

2.05%

GM2
0
0
0
10

3S193

82.2%

anti-GM2

71.2%

696

32.2%

ELISA
FACS
MCF-7
LSC

Pre
Post
Pre
Post
1:200
Pre
Post
1:200
CDC(MCF-7)

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
Mice #
Pre
Post

9. Heptavalent-
Tn
0
0
2560
40
10.51%
10.55%
84.31%
9.89%
60.45%
0.48%
10.40%
10.21%
92.22%
16.68%
63.24%
0.25%
9-1
−2.79%
34.02%

KLH +
Tf
0
0
5120
40

9-2
2.96%
9.42%

100 ug GPI (old
sTn
0
0
320
160

9-3
4.50%
11.41%

batch)
Muc1-G5
0
0
1280
0

9-4
6.74%
9.51%

(200 ul/mice)
Ley
0
0
40
320

9-5
4.01%
39.91%

globo H
0
80
0
320

3S193

97.83%

GM2
0
0
0
0

B72.3

5.34%

HMFG.1

3.01%

10. Heptavalent-
Tn
0
0
5120+
640
10.50%
10.44%
90.55%
12.59%
75.43%
0.27%
10.67%
10.24%
85.22%
11.17%
54.16%
0.74%
10-1
−6.29%
−3.3%

KLH +
Tf
0
0
5120
320

100 ug GPI-100 +
sTn
0
0
640
640

polysorbate 80
Muc1-G5
0
0
5120
80

(200 ul/mice)
Ley
0
0
0
320

globo H
0
160
20
1280

GM2
0
0
0
0

11. Heptavalent-
Tn
0
20
5120+
160
10.75%
10.39%
90.96%
4.8%
70.67%
0.23%
9.92%
10.74%
70.28%
8.33%
40.71%
0.29%
11-1
1.84%
10.93%

KLH +
Tf
0
80
5120+
640

11-2
0.71%
3.20%

10 ug QS-21
sTn
0
0
2560
320

11-3
1.31%
5.88%

(200 ul/mice)
Muc1-G5
0
0
2560
160

11-4
−1.58%
18.36%

Ley
0
0
10
10

11-5
10.28%
27.09%

globo H
0
80
40
640

GM2
0
0
0
0

12. Heptavalent-
Tn
0
0
1280
160
11.89%
10.49%
60.97%
3.33%
25.38%
0.23%
10.42%
10.29%
29.79%
4.55%
5.65%
0.14%

KLH +
Tf
0
0
1280
80

3 ug ER803022
sTn
0
0
80
80

(200 ul/mice)
Muc1-G5
0
0
80
20

Ley
0
0
0
20

globo H
20
160
80
640

GM2
0
0
0
0

13. Heptavalent-
Tn
0
20
160
160
10.59%
10.62%
60.86%
12.60%
15.51%
0.29%
10.50%
10.24%
45.30%
11.86%
5.60%
0.60%

KLH +
Tf
0
10
320
160

10 ug ER803732
sTn
0
40
20
160

(200 ul/mice)
Muc1-G5
0
0
160
80

Ley
0
0
0
80

globo H
20
80
80
320

GM2
0
0
0
0

14. 30 ug KLH +
Tn
0
0
0
160
10.62%
11.08%
11.02%
4.10%
5.61%
0.45%
10.32%
10.68%
9.09%
2.47%
7.96%
0.73%

100 ug GPI-100
Tf
0
40
0
320

(100 ul/mice)
sTn
0
0
0
80

Muc1-G5
0
10
0
160

Ley
0
0
0
0

globo H
0
160
10
640

GM2
0
0
0
160

KLH
0
10
5120++
320

Immunization of mice with Heptavalent-KLH Conjugates* plus QS-21 or GPI 100 with or without mAb 9H10 against CTLA-4.

Mean Value:

ELISA (mean)
ELISA (median)
FACS
MCF-7

custom-character

Pre
Post
Pre
Post
Pre
Post
1:200

custom-character

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
AVERAGE
MEDIAN

1. Heptavalent-KLH + 10 ug QS21
Tn
0
0
57440
640
0
0
25600
640
9.89%
9.78%
95.87%
77.77%
78.03%
16.09%
+CONTROL

Tf
0
0
10240++
260
0
0
10240+
160
9.39%
9.94%
96.40%
80.96%
79.70%
8.16%
VK-9
40.08%

sTn
0
0
3520
580
0
0
1280
320

MLS128
97.56%

Muc1-G5
0
0
1280
80
0
0
1280
80

antiGM2
####

Ley
0
32
1920
2560
0
0
1280
1280

MBr-1
####

globo H
0
48
672
128
0
80
640
160

GM2

2. Heptavalent-KLH + 100 ug
Tn
0
0
19200
840
0
0
25600
320
10.15%
10.36%
92.97%
79.87%
66.63%
28.35%

GPI100
Tf
0
0
10240+
260
0
0
10240+
160
10.10%
10.35%
95.99%
93.53%
69.88%
26.96%

sTn
0
0
720
360
0
0
320
80

Muc1-G5
0
0
1520
80
0
0
2560
160

Ley
0
0
3920
680
0
0
5120
640

globo H
0
0
320
176
0
0
80
160

GM2

3. Heptavalent-KLH + 100 ug GPI-
Tn
0
0
32000
480
0
0
25600
320
10.29%
10.14%
92.85%
62.94%
65.36%
18.34%

100 (Lyophilized)
Tf
0
0
10240+
340
0
0
10240+
320
10.20%
10.23%
92.35%
58.56%
63.59%
14.46%

sTn
0
0
1200
260
0
0
1280
320

Muc1-G5
0
0
1120
0
0
0
320
0

Ley
0
0
320
720
0
0
480
640

globo H
0
0
128
440
0
0
0
200

GM2

4. Heptavalent-KLH + 100 ug
Tn
0
0
38400
400
0
0
25600
160
10.14%
10.18%
91.34%
57.09%
70.79%
6.70%

GPI100′ + polysorbate80
Tf
0
0
10240+
140
0
0
10240+
160
10.22%
10.29%
90.80%
61.70%
67.27%
4.98%

sTn
0
0
1960
200
0
0
1280
320

Muc1-G5
0
0
4000
20
0
0
2560
0

Ley
0
0
1440
960
0
0
1280
640

globo H
0
40
100
224
0
40
120
160

GM2

5. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
61400
808
0
0
25600
640
9.92%
10.30%
89.55%
72.17%
64.38%
12.43%

Cytoxan 25 mg/Kg (I.P.) Day −1
Tf
0
0
10240++
560
0
0
10240++
640
10.19%
10.19%
90.87%
70.90%
66.42%
14.32%

sTn
0
0
520
480
0
0
640
320

Muc1-G5
0
0
3840
0
0
0
2560
0

Ley
0
0
480
200
0
0
0
80

globo H
0
0
32
540
0
0
0
400

6. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
32000
250
0
0
25600
160
10.33%
10.08%
90.59%
65.89%
62.40%
17.62%

mAb CTLA-4 in vaccine
Tf
0
0
10240+
1040
0
0
10240+
1280
10.26%
10.01%
91.50%
62.97%
63.04%
8.00%

(100 ug/mice) Day 0
sTn
0
0
6240
180
0
0
1280
200

Day 7& 14 no CTLA-4
Muc1-G5
0
0
1950
40
0
0
2560
40

Ley
0
0
180
2600
0
0
40
40

globo H
0
0
0
240
0
0
0
240

GM2

7. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
32000
1600
0
0
25600
1280
10.05%
10.31%
90.31%
85.42%
67.29%
29.21%

mAb CTLA-4 in vaccine
Tf
0
0
10240+
1920
0
0
10240+
1280
9.64%
10.41%
90.01%
85.58%
69.08%
21.26%

(100 ug/mice) Day 0 & 7
sTn
0
0
2880
100
0
0
2560
80

Day 14 no CTLA-4
Muc1-G5
0
0
6400
60
0
0
5120
80

Ley
0
0
32
208
0
0
0
160

globo H
0
0
32
220
0
0
0
240

GM2

8. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
85333
40
0
0
51200+
40
9.69%
10.15%
91.29%
45.33%
63.00%
6.19%

mAb CTLA-4 not in vaccine
Tf
0
0
10240++
370
0
0
10240++
320
9.63%
10.09%
90.20%
45.21%
50.05%
7.00%

I.P. day −1, 0, 1
sTn
0
0
480
0
0
0
640
0

Muc1-G5
0
0
3413
0
0
0
2560
0

Ley
0
0
320
106
0
0
160
0

globo H
0
0
53
240
0
0
0
80

GM2

9. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
56320
640
0
0
51200
640
10.25%
10.13%
93.16%
90.64%
73.15%
45.88%

Control mAb ROR-g2
Tf
0
0
10240+++
2720
0
0
10240+++
2560
10.27%
10.21%
94.17%
95.54%
76.62%
30.38%

100 ug/mice
sTn
0
0
3040
5200
0
0
1280
320

I.P. day −1, 0, 1
Muc1-G5
0
0
10240
160
0
0
10240
160

Ley
0
0
144
464
0
0
80
160

globo H
0
0
112
848
0
0
80
640

GM2

10. Heptavalent-KLH + 100 ug GPI100
Tn
0
0
81920
320
0
0
51200
160
10.42%
9.98%
88.03%
76.96%
67.02%
33.26%

100 ug/mice
Tf
0
0
10240++
920
0
0
10240++
320
10.50%
10.01%
87.97%
90.19%
64.58%
24.15%

sTn
0
0
2240
1440
0
0
2560
160

Muc1-G5
0
0
4160
40
0
0
2560
0

Ley
0
144
144
2640
0
160
80
320

globo H
0
0
0
224
0
0
0
160

GM2

Example 2
A Preclinical Study Comparing Approaches for Augmenting the Immunogenicity of a Heptavalent KLH-Conjugate Vaccine Against Epithelial Cancers

Previously using a series of monovalent vaccines, we have demonstrated that the optimal method for inducing an antibody response against cancer cell-surface antigens is covalent conjugation of the antigens to keyhole limpet hemocyanin (KLH) and the use of a saponin adjuvant. In preparation for testing a polyvalent (heptavalent)-KLH conjugate vaccine in the clinic, we have tested the impact on antibody induction against the 7 antigens of several variables described by others to augment immunogenicity. We explore here the impact of approaches for decreasing suppression of the immune response (low dose cyclophosphamide and anti-CTLA4 mAb), different saponin adjuvants (QS-21 and GPI-0100), and different methods of formulation (lyophilization and use of polysorbate 80). After two sets of experiments, these results are clear:

1) Immunization with the heptavalent-KLH conjugate vaccine induces high titers of antibodies against Tn (median ELISA titer IgM/IgG 320/10,240), sTn (640/2560), TF (320/5120), MUC1 (80/20,480) and globo H (1280/10), lower titers of antibodies against Lewis Y (160/80) and only occasional antibodies against GM2.

2) These antibodies reacted with the purified synthetic antigens by ELISA, and with naturally expressed antigens on the cancer cell surface by FACS.

3) Neither decreasing suppression with low dose cyclophosphamide or anti-CTLA4 mAb, nor changing the standard formulation by lyophilization or use of polysorbate 80 had any impact on antibody titers.

4) The two saponin adjuvants were comparably potent at our standard doses (QS-21 bug and GPI-0100 100 ug) but a third experiment comparing higher doses is in progress.

The high titers of antibodies against this heptavalent vaccine and the inability of these additional approaches to further augment antibody titers confirms that the combination of conjugation to KLH and use of a saponin adjuvant is sufficiently optimized for testing in the clinic.

There is a broad and expanding body of pre-clinical and clinical studies demonstrating that naturally acquired, actively induced, and passively administered antibodies are able to eliminate circulating tumor cells and micro metastases (1). Induction of antibodies against tumor antigens is more difficult than induction of antibodies against viral and bacterial antigens because most tumor antigens are normal or slightly modified auto antigens and because actively growing tumors may set in motion mechanisms which suppress the anti-cancer cell immune response. Consequently it may be necessary to overcome not only some level of tolerance but also some additional level of active suppression, making the immunization approach critical. We have previously reported that the optimal approach for induction of antibodies against gangliosides and a variety of other carbohydrate and peptide antigens is covalent attachment of the tumor antigen to an immunogenic carrier molecule (keyhole limpet hemocyanin (KLH) was optimal (2,3)) plus the use of a potent immunological adjuvant. In our previous experience saponin adjuvants such as QS-21 and GPI-0100 were the optimal adjuvants (4,5).

In preparation for clinical trials with a heptavalent KLH-conjugate vaccine we test here the impact of several variables including 1) vaccine formulation (lyophilization or the use of polysorbate 80), 2) decreasing suppression (low dose cyclophosphamide or anti-CTLA4 mAb), or 3) various doses of the two saponin adjuvants QS-21 and GPI-0100, on antibody titers against the individual antigens and tumor cells expressing these antigens.

Pathogen-free female BALB/c or C57BL/6 mice 6-10 weeks of age were obtained from the Jackson Laboratory (Bar Harbor, Me.). QS-21 was obtained from Aquila Biopharmaceuticals (Framingham, Mass. (now Antigenics Inc., NYC, NY)), GPI-0100 was obtained from Galenica Pharmaceuticals, Inc. (Birmingham, Ala.). Cytoxan (25 mg/kg) was purchased and injected IP one day prior to the first immunization. The hybridoma for murine monoclonal antibody CTLA-4 was obtained from Jim Allison (Berkeley, Calif.) and the mAb was prepared by Dr. Polly Gregor (MSKCC). The reactivity of mAb with CTLA-4 was confirmed. Polysorbate 80 was purchased.

Immunization of Mice:

Groups of five mice were immunized 3 times at one week intervals with the heptavalent vaccine containing 3 mcg of each of the 7 antigens covalently conjugated to KLH and mixed with GPI-0100 or QS-21 as indicated. Vaccines were administered subcutaneously over the lower abdomen. A 4th, booster, immunization was given at week 8.

Serological Assays:

For the ELISA assay, glycosylated MUC1, globo H, Lewis Y or GM2, or Tn, sTn or TF conjugated to BSA, were coated on ELISA plates at an antigen dose of 0.1-0.2 mcg per well.

Phosphatase-conjugated goat anti-mouse IgG or IgM was added at a dilution of 1:200 (Southern Biotechnology Associates, Inc., Birmingham, Ala.). Antibody titer was the highest dilution yielding absorbance of 0.10 or greater.

F ACS Analysis:

MCF-7 human breast cancer cells expressing all seven antigens but especially Lewis Y and MUC1 and sTn, and LSC expressing especially Lewis Y, sTn and Tn, were used. Single cell suspensions of 5×10⁷cells/tube were washed in PBS with 3% fetal calf serum and incubated with 20 mcl of full strength or 1/200 diluted antisera for 30 minutes on ice. 20 microliters of 1/15 goat anti-mouse IgG or IgM labeled with FITC were all added and percent positive cells and mean fluorescent intensity (MFI) of stained cells analyzed using a F ACScan (Becton Dickenson, Calif.). Pre and post vaccination sera were analyzed together and the pre-treatment percent positive cells set at 10%.

Comparison of the Immune Response after Immunization with Monovalent and Hexavalent-KLH Conjugate Vaccines Against Prostate Cancer

Glycolipid and glycoprotein differentiation antigens such as GM2, Globo H, Lewis y, Tn, TF, and mucin 1 (MUC1) are over-expressed on the cell surface of many tumors. Of the many approaches to immunization we have tested, covalent conjugation of antigens such as these to keyhole limpet hemocyanin (KLH) plus the use of immunological adjuvant QS-21 has been the optimal approach for inducing IgM and IgG antibodies. Immunization of patients with monovalent vaccines containing these antigens has demonstrated the consistent immunogenicity and safety of these vaccines. However, to overcome the heterogeneous nature of tumors, and of the immune response in different individuals, we have recently vaccinated a small group of patients (prostate cancer with rising PSA, but free of detectable disease) with a hexavalent-KLH vaccine containing GM2, Globo H, Le^y, Tn(c), TF(c) and glycosylated MUC1 individually conjugated with KLH and mixed with immunological adjuvant QS-21. The main objective of this presentation is to compare the immune response of the six initial patients receiving hexavalent vaccine with the immune responses of patients who had previously been immunized with the respective monovalent vaccines. All patients were vaccinated six times (weeks 1,2,3,7,19 and 31) and bloods obtained pre treatment and on weeks 7 and 9 were tested at one time. RECIPRICOL MEAN PEAK ELISA TITER AFTER IMMUNIZATION IgM/IgG.

Antigen

Globo

GM2
H
Le^y
Tn
TF
MUC1

Polyvalent
Pending
160/0
0/0
640/640
1280/160
40/320

vaccine

Individual
Pending
160/0
0/10
1280/2560
1280/160
2560/320

Vaccine

Because of the low response against Le^y, we are continuing studies aimed at creating a more immunogenic Le^yvaccine. Comparing the responses induced by monovalent and hexavalent vaccines, there was no significant difference in the antibody responses against any of the five antigens tested to date. Combination of six individual conjugates into a single vaccine does not significantly change the antibody response against the individual antigens.

Experiment 1: Median ELISA titers and FACS results after vaccination

of groups of 5 Balb/c mice with Heptavalent-KLH conjugate

ELISA(mean)
ELISA(median)

Pre
Post
Pre
Post

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM

1. Heptavalent-KLH +
Tn
0
0
57440
640
0
0
25600
640

10 ug QS21
Tf
0
0
10240++
260
0
0
10240+
160

sTn
0
0
3520
580
0
0
1280
320

Muc1-G5
0
0
1280
80
0
0
1280
80

Ley
0
32
1920
2560
0
0
1280
1280

globo H
0
48
672
128
0
80
640
160

GM2

2. Heptavalent-KLH +
Tn
0
0
19200
840
0
0
25600
320

100 ug GPI100
Tf
0
0
10240+
260
0
0
10240+
160

sTn
0
0
720
360
0
0
320
80

Muc1-G5
0
0
1520
80
0
0
2560
160

Ley
0
0
3920
680
0
0
5120
640

globo H
0
0
320
176
0
0
80
160

GM2

3. Heptavalent-KLH +
Tn
0
0
32000
480
0
0
25600
320

100 ug GPI-100
Tf
0
0
10240+
340
0
0
10240+
320

(Lyophilized)
sTn
0
0
1200
260
0
0
1280
320

Muc1-G5
0
0
1120
0
0
0
320
0

Ley
0
0
320
720
0
0
480
640

globo H
0
0
128
440
0
0
0
200

GM2

4. Heptavalent-KLH +
Tn
0
0
38400
400
0
0
25600
160

100 ug GPI100′ +
Tf
0
0
10240+
140
0
0
10240+
160

polysorbate80
sTn
0
0
1960
200
0
0
1280
320

Muc1-G5
0
0
4000
20
0
0
2560
0

Ley
0
0
1440
960
0
0
1280
640

globo H
0
40
100
224
0
40
120
160

GM2

5. Heptavalent-KLH +
Tn
0
0
61400
808
0
0
25600
640

100 ug GPI100
Tf
0
0
10240++
560
0
0
10240++
640

Cytoxan 25 mg/Kg
sTn
0
0
520
480
0
0
640
320

(I.P.) Day −1
Muc1-G5
0
0
3840
0
0
0
2560
0

Ley
0
0
480
200
0
0
0
80

globo H
0
0
32
540
0
0
0
400

GM2

6. Heptavalent-KLH +
Tn
0
0
32000
250
0
0
25600
160

100 ug GPI100
Tf
0
0
10240+
1040
0
0
10240+
1280

mAb CTLA-4 in
sTn
0
0
6240
180
0
0
1280
200

vaccine
Muc1-G5
0
0
1950
40
0
0
2560
40

(100 ug/mice) Day 0
Ley
0
0
180
2600
0
0
40
40

Day 7& 14 no
globo H
0
0
0
240
0
0
0
240

CTLA-4
GM2

7. Heptavalent-KLH +
Tn
0
0
32000
1600
0
0
25600
1280

100 ug GPI100
Tf
0
0
10240+
1920
0
0
10240+
1280

mAb CTLA-4 in
sTn
0
0
2880
100
0
0
2560
80

vaccine
Muc1-G5
0
0
6400
60
0
0
5120
80

(100 ug/mice) Day 0
Ley
0
0
32
208
0
0
0
160

& 7
globo H
0
0
32
220
0
0
0
240

Day 14 no CTLA-4
GM2

8. Heptavalent-KLH +
Tn
0
0
85333
40
0
0
51200+
40

100 ug GPI100
Tf
0
0
10240++
370
0
0
10240++
320

mAb CTLA-4 not in
sTn
0
0
480
0
0
0
640
0

vaccine
Muc1-G5
0
0
3413
0
0
0
2560
0

I.P. day −1, 0, 1
Ley
0
0
320
106
0
0
160
0

globo H
0
0
53
240
0
0
0
80

GM2

Pre

Post

Pre

Post

9. Heptavalent-KLH +
Tn
0
0
56320
640
0
0
51200
640

100 ug GPI100
Tf
0
0
10240+++
2720
0
0
10240+++
2560

Control mAb ROR-g2
sTn
0
0
3040
5200
0
0
1280
320

100 ug/mice
Muc1-G5
0
0
10240
160
0
0
10240
160

I.P. day −1, 0, 1
Ley
0
0
144
464
0
0
80
160

globo H
0
0
112
848
0
0
80
640

GM2

10. Heptavalent-KLH +
Tn
0
0
81920
320
0
0
51200
160

100 ug GPI100
Tf
0
0
10240++
920
0
0
10240++
320

100 ug/mice
sTn
0
0
2240
1440
0
0
2560
160

Muc1-G5
0
0
4160
40
0
0
2560
0

Ley
0
144
144
2640
0
160
80
320

globo H
0
0
0
224
0
0
0
160

GM2

FACS MCF-7

Pre
Post
1:200

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
+CONTROL

1. Heptavalent-KLH +
Tn
10%
10%
96%
78%
78%
16%
VK-9
40.08%

10 ug QS21
Tf
9%
10%
96%
81%
80%
8%
MLS128
97.56%

sTn

antiGM2
98.87%

Muc1-G5

MBr-1
58.06%

Ley

globo H

GM2

2. Heptavalent-KLH +
Tn
10%
10%
93%
80%
67%
28%

100 ug GPI100
Tf
10%
10%
96%
94%
70%
27%

sTn

Muc1-G5

Ley

globo H

GM2

3. Heptavalent-KLH +
Tn
10%
10%
93%
63%
65%
18%

100 ug GPI-100
Tf
10%
10%
92%
59%
64%
14%

(Lyophilized)
sTn

Muc1-G5

Ley

globo H

GM2

4. Heptavalent-KLH +
Tn
10%
10%
91%
57%
71%
7%

100 ug GPI100′ +
Tf
10%
10%
91%
62%
67%
5%

polysorbate80
sTn

Muc1-G5

Ley

globo H

GM2

5. Heptavalent-KLH +
Tn
10%
10%
90%
72%
64%
12%

100 ug GPI100
Tf
10%
10%
91%
71%
66%
14%

Cytoxan 25 mg/Kg
sTn

(I.P.) Day −1
Muc1-G5

Ley

globo H

GM2

6. Heptavalent-KLH +
Tn
10%
10%
91%
66%
62%
18%

100 ug GPI100
Tf
10%
10%
92%
63%
63%
8%

mAb CTLA-4 in
sTn

vaccine
Muc1-G5

(100 ug/mice) Day 0
Ley

Day 7& 14 no
globo H

CTLA-4
GM2

7. Heptavalent-KLH +
Tn
10%
10%
90%
85%
67%
29%

100 ug GPI100
Tf
10%
10%
90%
86%
69%
21%

mAb CTLA-4 in
sTn

vaccine
Muc1-G5

(100 ug/mice) Day 0
Ley

& 7
globo H

Day 14 no CTLA-4
GM2

8. Heptavalent-KLH +
Tn
10%
10%
91%
45%
63%
6%

100 ug GPI100
Tf
10%
10%
90%
45%
50%
7%

mAb CTLA-4 not in
sTn

vaccine
Muc1-G5

I.P. day −1, 0, 1
Ley

globo H

GM2

9. Heptavalent-KLH +
Tn
10%
10%
93%
91%
73%
46%

100 ug GPI100
Tf
10%
10%
94%
96%
77%
30%

Control mAb ROR-g2
sTn

100 ug/mice
Muc1-G5

I.P. day −1, 0, 1
Ley

globo H

GM2

10. Heptavalent-KLH +
Tn
10%
10%
88%
77%
67%
33%

100 ug GPI100
Tf
11%
10%
88%
90%
65%
24%

100 ug/mice
sTn

Muc1-G5

Ley

globo H

GM2

Experiment 2: Median ELISA titers and FACS results against MCF-7 and LSC cells after

vaccination groups of 5 C57BL/6 Mice with heptavalent-KLH conjugate vaccine

FACS

ELISA
withMCF-7

Pre
Post
Pre
Post

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM

Heptavalent-KLH +
Tn
0
10
5120+
320
10%
11%
91.61%
18.46%

100 ug GPI100
Tf
0
10
5120
320

99%
24%

(200 ul/mice)
sTn
0
0
2560
640

Muc1-G5
0
0
5120++
80

Ley
0
0
80
160

globo H
0
80
10
1280

GM2
0
0
0
10

Heptavalent-KLH +
Tn
0
0
2560
40
11%
11%
84.31%
9.89%

100 ug GPI (old
Tf
0
0
5120
40

batch)
sTn
0
0
320
160

(200 ul/mice)
Muc1-G5
0
0
1280
0

Ley
0
0
40
320

globo H
0
80
0
320

GM2
0
0
0
0

Heptavalent-KLH +
Tn
0
0
5120+
640
11%
10%
90.55%
12.59%

100 ug GPI-100 +
Tf
0
0
5120
320

polysorbate 80
sTn
0
0
640
640

(200 ul/mice)
Muc1-G5
0
0
5120
80

Ley
0
0
0
320

globo H
0
160
20
1280

GM2
0
0
0
0

Heptavalent-KLH +
Tn
0
20
5120+
160
11%
10%
90.96%
4.8%

10 ug QS-21
Tf
0
80
5120+
640

(200 ul/mice)
sTn
0
0
2560
320

Muc1-G5
0
0
2560
160

Ley
0
0
10
10

globo H
0
80
40
640

GM2
0
0
0
0

Heptavalent-KLH +
Tn
0
20
160
160
11%
11%
60.86%
12.60%

10 ug
Tf
0
10
320
160

ER803732
sTn
0
40
20
160

200 ul/mice)
Muc1-G5
0
0
160
80

Ley
0
0
0
80

globo H
20
80
80
320

GM2
0
0
0
0

FACS
FACS with LSC

withMCF-7
# LSC

1:200
Pre
Post
1:200

Group #
Antigen
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM

Heptavalent-KLH +
Tn
80%
18%
10%
11%
96.04%
39.25%
84%
39%

100 ug GPI100
Tf
82%
21%

(200 ul/mice)
sTn

Muc1-G5

Ley

globo H

GM2

Heptavalent-KLH +
Tn
60%
10%
10%
10%
92.22%
16.68%
63%
17%

100 ug GPI (old
Tf

batch)
sTn

(200 ul/mice)
Muc1-G5

Ley

globo H

GM2

Heptavalent-KLH +
Tn
75%
13%
11%
10%
85.22%
11.17%
54%
11%

100 ug GPI-100 +
Tf

polysorbate 80
sTn

(200 ul/mice)
Muc1-G5

Ley

globo H

GM2

Heptavalent-KLH +
Tn
71%
5%
10%
11%
70.28%
8.33%
41%
8%

10 ug QS-21
Tf

(200 ul/mice)
sTn

Muc1-G5

Ley

globo H

GM2

Heptavalent-KLH +
Tn
16%
13%
11%
10%
45.30%
11.86%
6%
12%

10 ug
Tf

ER803732
sTn

200 ul/mice)
Muc1-G5

Ley

globo H

GM2

col 00-106:

Pilot Phas text missing or illegible when filed

Trial: Vaccination of Patients Who Have Ovarian, Fallopian Tube or Peritoneal Cancer with A Polyvalent Vaccine-KLH Conjugate + QS-21

Patient Name
Vaccine:

Pa-

10 ug GM2
10 ug Globo-H
10 ug LeY

tient

Muc1-1G5
Globo-H
LeY

#
Vaccination
Serology
Sera #
IgM
IgG
IgM
IgG
IgM
IgG

Jun. 12, 2002
Jun. 12, 2002
Jun. 27, 2002
Jun. 19, 2002
Jun. 21, 2002
Jun. 21, 2002

Pa-
Jul. 03, 2001
Jul. 03, 2001
P7OVQ
0
0
0
0
0
0

tient

2

1
Jul. 10, 2001
Jul. 31, 2001
P7OVQ
2560
640
40
0
0
0

6

Jul. 17, 2001
Aug. 14, 2001
P7OVQ
2560
640
40
0
0
0

9

Aug. 14, 2001
Aug. 08, 2001
P7OVQ
2560
320
40
0
0
0

15

OFF TRIAL

(+)

Control

M62
2560
640

Positve

2560

control

S193(1

6400

mg/ml)

Positve

2560

control

Positve

control

Positve

control

Positve

control

Positve

2560

control

Jun. 04, 2002
Jun. 04, 2002
Jun. 27, 2002
Jun. 26, 2002

Pa-
Jul. 03, 2001
Jul. 03, 2001
P7OVQ
0
0
0
0

tient

3

2
Jul. 10, 2001
Jul. 31, 2001
P7OVQ
80
20
0
0

7

Jul. 17, 2001
Aug. 14, 2001
P7OVQ
40
20
0
0

10

Aug. 14, 2001
Aug. 28, 2001
P7OVQ
20
40
0
0

13

Sep. 25, 2001
P7OVQ
20
20
0
0

20

Oct. 09, 2001
Oct. 09, 2001
P7OVQ
20
20
0
0

24

Oct. 23, 2001
P7OVQ
20
20
0
0

30

Jan. 11, 2002
P7OVQ
0
0
0
0

49

Jun. 07, 2002
P7OVQ

0
0

65

(+)

Control

Positve
2560
640

control

Positve

2560

control

Positve

640

control

Patient Name
Vaccine:

Pa-
3 ug Muc1G5
3 ug Tn(c)
3 ug S-Tn(c)
3 ug TF(c)

tient
GM2
Tn(c)
S-Tn(c)
TF(c)

#
Vaccination
Serology
Sera #
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG

Jun. 24, 2002
Jun. 24, 2002

Jun. 25, 2002
Jun. 25, 2002

Pa-
Jul. 03, 2001
Jul. 03, 2001
P7OVQ
0
0

0
20

tient

2

1
Jul. 10, 2001
Jul. 31, 2001
P7OVQ
0
20

1280
160

6

Jul. 17, 2001
Aug. 14, 2001
P7OVQ
0
20

1280
160

9

Aug. 14, 2001
Aug. 09, 2001
P7OVQ
0
20

1280
320

15

OFF TRIAL

(+)

Control

M62

Positve

control

S193(1

mg/ml)

Positve

control

Positve
640

control

Positve

2560

control

Positve

2560
2560

control

Positve

control

Pa-
Jul. 03, 2001
Jul. 03, 2001
P7OVQ

tient

3

2
Jul. 10, 2001
Jul. 31, 2001
P7OVQ

7

Jul. 17, 2001
Aug. 14, 2001
P7OVQ

10

Aug. 14, 2001
Aug. 28, 2001
P7OVQ

13

Sep. 25, 2001
P7OVQ

20

Oct. 09, 2001
Oct. 09, 2001
P7OVQ

24

Oct. 23, 2001
P7OVQ

30

Jan. 11, 2002
P7OVQ

49

Jun. 07, 2002
P7OVQ

65

(+)

Control

Positve

control

Positve

control

Positve

control

Patient Name

Med-

ical
Muc1-1G5
Globo-H
LeY

#
Vaccination
Serology
Sera #
IgM
IgG
IgM
IgG
IgM
IgG

Jun. 07, 2002
Jun. 07, 2002
Jun. 27, 2002
Jun. 26, 2002

Pa-
Jul. 10, 2001
Jul. 10, 2001
P7OVQ
0
0
20
0

tient

4

3
Jul. 17, 2001
Aug. 07, 2001
P7OVQ
1280
160
160
0

8

Jul. 24, 2001
Aug. 21, 2001
P7OVQ
320
40
80
0

12

Aug. 21, 2001
Sep. 04, 2001
P7OVQ
160
80
80
0

18

Oct. 02, 2001
P7OVQ
80
40
40
0

22

Oct. 16, 2001
Oct. 16, 2001
P7OVQ
40
40
80
0

26

Oct. 30, 2001
P7OVQ
80
80
40
0

33

Jan. 08, 2002
P7OVQ
40
40
80
0

47

(+)

Control

M62
2560
1280

Positve

2560

control

Positve

1280

control

Jun. 10, 2002
Jun. 10, 2002

pa-
Jul. 24, 2001
Jul. 24, 2001
P7OVQ
0
0

tient

5

4
Jul. 31, 2001
Aug. 21, 2001
P7OVQ
1280
80

14

Aug. 07, 2001
Sep. 04, 2001
P7OVQ
1280
40

17

Sep. 04, 2001
Sep. 18, 2001
P7OVQ
160
20

23

Oct. 16, 2001
P7OVQ
160
20

27

Oct. 30, 2001
Oct. 30, 2001
P7OVQ
80
40

32

Nov. 13, 2001
P7OVQ
20
20

36

Jan. 22, 2002
P7OVQ
20
20

52

Mar. 26, 2002
P7OVQ
20
20

63

(+)

Control

M62
1280
640

Jun. 12, 02
Jun. 12, 02
Jun. 27, 2002
Jun. 19, 2002
Jun. 21, 2002
Jun. 21, 2002

pa-
Aug. 16, 2001
Aug. 16, 2001
P7OVQ
0
0
0
0
0
0

tient

11

5
Aug. 23, 2001
Sep. 27, 2001
P7OVQ
80
80
0
0
0
0

21

Aug. 30, 2001
Oct. 11, 2001
P7OVQ
40
80
0
0
0
0

25

Sep. 27, 2001
OFF TRIAL

(+)

Control

M62
2560
640

Positve

2560

control

S193(1

6400

mg/ml)

Positve

2560

control

Positve

control

Positve

control

Positve

control

Positve

2560

control

Jun. 17, 2002
Jun. 17, 2002

Pa-
Aug. 30, 2001
Aug. 30, 2001
P7OVQ
0
0

tient

16

6
Sep. 06, 2001
Sep. 27, 2001
P7OVQ
160
20

19

Sep. 13, 2001
Oct. 25, 2001
P7OVQ
40
20

31

Oct. 11, 2001
Nov. 22, 2001
P7OVQ
20
0

39

Dec. 06, 2001
Dec. 06, 2001
P7OVQ
20
0

41

Dec. 20, 2001
P7OVQ
20
20

44

Mar. 08, 2002
P7OVQ
20
20

62

(+)

Control

M62
2560
320

Jun. 13, 2002
Jun. 13, 2002
Jun. 27, 2002
Jun. 19, 2002
Jun. 21, 2002
Jun. 21, 2002

pa-
Oct. 19, 2001
Oct. 19, 2001
P7OVQ
0
0
0
(re-do)
0
0

tient

28

7
Oct. 26, 2001
Nov. 16, 2001
P7OVQ
640
40
0
(re-do)
0
0

35

Nov. 02, 2001
Dec. 14, 2001
P7OVQ
80
20
0
(re-do)
0
0

42

Nov. 30, 2001
Jan. 11, 2002
P7OVQ
80
20
0
(re-do)
0
0

48

Jan. 25, 2002
Jan. 25, 2002
P7OVQ
80
20
0
(re-do)
0
0

53

Feb. 08, 2002
P7OVQ
80
20
0
(re-do)
0
0

56

Apr. 19, 2002

(+)

Control

M62
2560
160

Positve

2560

control

S193(1

6400

mg/ml)

Positve

2560

control

Positve

control

Positve

control

Positve

control

Positve

2560

control

Jun. 18, 2002
Jun. 18, 2002

Pa-
Oct. 23, 2001
Oct. 23, 2001
P7OVQ
0
0

tient

29

8
Oct. 30, 2001
Nov. 20, 2001
P7OVQ
0
0

38

Nov. 06, 2001
Dec. 18, 2001
P7OVQ
0
0

43

Dec. 04, 2001
Jan. 15, 2002
P7OVQ
0
0

51

Jan. 29, 2002
Jan. 29, 2002
P7OVQ
40
0

54

OFF TRIAL

(+)

Control

M62
2560
640

Jun. 18, 2002
Jun. 18, 2002

Pa-
Nov. 06, 2001
Nov. 06, 2001
P7OVQ
0
0

tient

34

9
Nov. 13, 2001
Dec. 04, 2001
P7OVQ
1280
80

40

Nov. 20, 2001
Jan. 01, 2002
P7OVQ
320
80

45

Dec. 18, 2001
Jan. 29, 2002
P7OVQ
320
80

55

Feb. 12, 2002
Feb. 12, 2002
P7OVQ
160
40

58

Feb. 26, 2002
P7OVQ
160
80

60

May 09, 2002
P7OVQ
40
80

64

(+)

Control

M62
2560
320

Jun. 13, 2002
Jun. 13, 2002
Jun. 27, 2002
Jun. 19, 2002
Jun. 21, 2002
Jun. 21, 2002

Pa-
Nov. 20, 2001
Nov. 20, 2001
P7OVQ
0
0
0
(re-do)
0
0

tient

37

10
Nov. 27, 2001
Dec. 18, 2001
P7OVQ
320
80
320
(re-do)
0
20

46

Dec. 04, 2001
Jan. 15, 2002
P7OVQ
320
320
320
(re-do)
0
20

50

Jan. 01, 2002
Feb. 12, 2002
pt no
—
—
—
—
—
—

show

Feb. 26, 2002
Feb. 26, 2002
P7OVQ
40
160
80
(re-do)
0
20

59

Mar. 12, 2002
pt no
—
—
—
—
—
—

show

May 21, 2002
pt no
—
—
—
—
—
—

show

(+)

Control

M62
2560
160

Positve

2560

control

S193(1

6400

mg/ml)

Positve

2560

control

Positve

control

Positve

control

Positve

control

Positve

1280

control

Jun. 12, 2002
Jun. 12, 2002
Jun. 27, 2002
Jun. 19, 2002
Jun. 21, 2002
Jun. 21, 2002

Pa-
Mar. 07, 2001
Mar. 07, 2001
P7OVQ
0
0
0
0
0
0

tient

1

11
Feb. 05, 2002
Feb. 05, 2001
P7OVQ
0
0
0
0
0
0

57

Feb. 12, 2002
Mar. 05, 2002
P7OVQ
0
20
0
0
0
0

61

Feb. 19, 2002
OFF TRIAL

Mar. 19, 2002

(+)

Control

M62
2560
640

Positve

2560

control

S193(1

6400

mg/ml)

Positve

2560

control

Positve

control

Positve

control

Positve

control

Positve

2560

control

Patient Name

Med-

ical
GM2
Tn(c)
STn(c)
Tf

#
Vaccination
Serology
Sera #
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG

Pa-
Jul. 10, 2001
Jul. 10, 2001
P7OVQ

tient

4

3
Jul. 17, 2001
Aug. 07, 2001
P7OVQ

8

Jul. 24, 2001
Aug. 21, 2001
P7OVQ

12

Aug. 21, 2001
Aug. 04, 2001
P7OVQ

18

Oct. 02, 2001
P7OVQ

22

Oct. 16, 2001
Oct. 16, 2001
P7OVQ

26

Oct. 30, 2001
P7OVQ

33

Jan. 08, 2002
P7OVQ

47

(+)

Control

M62

Positve

control

Positve

control

pa-
Jul. 24, 2001
Jul. 24, 2001
P7OVQ

tient

5

4
Jul. 31, 2001
Aug. 21, 2001
P7OVQ

14

Aug. 07, 2001
Sep. 04, 2001
P7OVQ

17

Sep. 04, 2001
Aug. 18, 2001
P7OVQ

23

Oct. 16, 2001
P7OVQ

27

Oct. 30, 2001
Oct. 30, 2001
P7OVQ

32

Nov. 13, 2001
P7OVQ

36

Jan. 22, 2002
P7OVQ

52

Mar. 26, 2002
P7OVQ

63

(+)

Control

M62

Jun. 24, 2002
Jun. 24, 2002

Jun. 25, 2002
Jun. 25, 2002

pa-
Aug. 16, 2001
Aug. 16, 2001
P7OVQ
0
0

0
0

tient

11

5
Aug. 23, 2001
Sep. 27, 2001
P7OVQ
0
0

40
160

21

Aug. 30, 2001
Oct. 11, 2001
P7OVQ
0
0

0
160

25

Sep. 27, 2001
OFF TRIAL

(+)

Control

M62

Positve

control

S193(1

mg/ml)

Positve

control

Positve
640

control

Positve

2560

control

Positve

2560
2560

control

Positve

control

Pa-
Aug. 30, 2001
Aug. 30, 2001
P7OVQ

tient

16

6
Sep. 06, 2001
Sep. 27, 2001
P7OVQ

19

Sep. 13, 2001
Oct. 25, 2001
P7OVQ

31

Oct. 11, 2001
Nov. 22, 2001
P7OVQ

39

Dec. 06, 2001
Dec. 06, 2001
P7OVQ

41

Dec. 20, 2001
P7OVQ

44

Mar. 08, 2002
P7OVQ

62

(+)

Control

M62

Jun. 24, 2002
Jun. 24, 2002

Jun. 25, 2002
Jun. 25, 2002

pa-
Oct. 19, 2001
Oct. 19, 2001
P7OVQ
0
0

20
0

tient

28

7
Oct. 26, 2001
Nov. 16, 2001
P7OVQ
0
0

160
160

35

Nov. 02, 2001
Dec. 14, 2001
P7OVQ
0
0

80
160

42

Nov. 30, 2001
Jan. 11, 2002
P7OVQ
0
20

80
80

48

Jan. 25, 2002
Jan. 25, 2002
P7OVQ
0
20

80
40

53

Feb. 08, 2002
P7OVQ
0
20

80
80

56

Apr. 19, 2002

(+)

Control

M62

Positve

control

S193(1

mg/ml)

Positve

control

Positve
640

control

Positve

2560

control

Positve

2560
2560

control

Positve

control

Pa-
Oct. 23, 2001
Oct. 23, 2001
P7OVQ

tient

29

8
Oct. 30, 2001
Nov. 20, 2001
P7OVQ

38

Nov. 06, 2001
Dec. 18, 2001
P7OVQ

43

Dec. 04, 2001
Jan. 15, 2002
P7OVQ

51

Jan. 29, 2002
Jan. 29, 2002
P7OVQ

54

OFF TRIAL

(+)

Control

M62

Pa-
Nov. 06, 2001
Nov. 06, 2001
P7OVQ

tient

34

9
Nov. 13, 2001
Dec. 04, 2001
P7OVQ

40

Nov. 20, 2001
Jan. 01, 2002
P7OVQ

45

Dec. 18, 2001
Jan. 29, 2002
P7OVQ

55

Feb. 12, 2002
Feb. 12, 2002
P7OVQ

58

Feb. 26, 2002
P7OVQ

60

May 09, 2002
P7OVQ

64

(+)

Control

M62

Jun. 24, 2002
Jun. 24, 2002

Jun. 25, 2002
Jun. 25, 2002

Pa-
Nov. 20, 2001
Nov. 20, 2001
P7OVQ
0
0

0
0

tient

37

10
Nov. 27, 2001
Dec. 18, 2001
P7OVQ
0
20

160
80

46

Dec. 04, 2001
Jan. 15, 2002
P7OVQ
0
20

80
640

50

Jan. 01, 2002
Feb. 12, 2002
pt no
—
—

—
—

show

Feb. 26, 2002
Feb. 26, 2002
P7OVQ
0
20

40
320

59

Mar. 12, 2002
pt no
—
—

—
—

show

May 21, 2002
pt no
—
—

—
—

show

(+)

Control

M62

Positve

control

S193(1

mg/ml)

Positve

control

Positve
640

control

Positve

2560

control

Positve

2560
2560

control

Positve

control

Jun. 24, 2002
Jun. 24, 2002

Jun. 25, 2002
Jun. 25, 2002

Pa-
Mar. 07, 2001
Mar. 07, 2001
P7OVQ
0
20

20
0

tient

1

11
Feb. 05, 2002
Feb. 05, 2001
P7OVQ
0
0

20
0

57

Feb. 12, 2002
Mar. 05, 2002
P7OVQ
0
0

40
80

61

Feb. 19, 2002
OFF TRIAL

Mar. 19, 2002

(+)

Control

M62

Positve

control

S193(1

mg/ml)

Positve

control

Positve
640

control

Positve

2560

control

Positve

2560
2560

control

Positve

control

* Patient received one vaccine before protocol hold, restarted ~1 year later

text missing or illegible when filed

indicates data missing or illegible when filed

Protocol # 01-019: Serological analysis of Breast cancer patient vaccinated with hexavalent vaccine

ELISA GM2
ELISA MUC-1-1
ELISA LeY Ceramide
ELISA Globo H

(10 mcg)(March
5G (3
(10 mcg)
Ceramide(10

Vaccine
Sample

2002)
mcg)(March 2002)
(April 2002)
mcg) (May 2002)

Patient #
Date
Date
Serology Top
IgG
IgM
IgG
IgM
IgG
IgM
IgG

Patient
Jan. 16, 2002
Jan. 16, 2002
P7BRQ4
20
0
0
0
0
0
0

1
Jan. 23, 2002
Jan. 23, 2002
P7BRQ9
0
0
0
0
0
0
0

Jan. 30, 2002
Jan. 30, 2002
P7BRQ11
0
0
0
0
0
0
0

Feb. 13, 2002
P7BRQ19
0
0
40
80
0
0
0

Feb. 27, 2002
Feb. 27, 2002
P7BRQ28
0
0
20
80
0
0
0

Mar. 13, 2002
P7BRQ37
0
40
40
80
0
0
0

Apr. 10, 2002
P7BRQ44

80
320
0
0
0

May 22, 2002
May 22, 2002
P7BRQ62

Jun. 05, 2002
P7BRQ67

Controls

>2560

320

(M62)

320

2560

(MCG170)

160

2560

(LeYM12)

20

80/160

Mono Ab (S193)

1280

(GB81)

0

Mono Ab (VK9)

5120

(P7BRQ17)

(slovin lab wk 7)

Patient
Jan. 16, 2002
Jan. 16, 2002
P7BRQ5
0
0
0
0
0
0
0

2
Jan. 23, 2002
Jan. 23, 2002
P7BRQ8
0
0
0
0
0
0
0

Jan. 30, 2002
Jan. 30, 2002
P7BRQ12
0
0
0
0
0
0
0

Feb. 13, 2002
P7BRQ20
0
0
80
160
0
0
0

Feb. 27, 2002
Feb. 27, 2002
P7BRQ27
0
80
40
20
0
0
0

Mar. 13, 2002
P7BRQ36
0
160
80
20
0
0
0

Apr. 10, 2002
P7BRQ46

80
80
0
0
0

May 22, 2002
May 22, 2002
P7BRQ61

Jun. 05, 2002
P7BRQ68

Controls

>2560

320

(P7BRQ17)

>2560

(hexavalent)

80

320

(P7BRQ16)

640

(LeYM12)

0

160

Mono Ab (S193)

1280

(GB81)

0

Mono Ab (VK9)

5120

(P7BRQ17)

(slovin lab wk 7)

Patient
Jan. 07, 2002
Jan. 07, 2002
P7BRQ1
0
0
0
0
0
0
0

3
Jan. 14, 2002
Jan. 14, 2002
P7BRQ3
0
0
0
0
0
0
0

Jan. 21, 2002
Jan. 21, 2002
P7BRQ7
0
0
0
320
0
20
0

Feb. 04, 2002
P7BRQ17
0
20
80
2560
0
40
0

Feb. 18, 2002
Feb. 18, 2002
P7BRQ23
0
0
80
640
0
20
0

Mar. 04, 2002
P7BRQ30
0
0
80
320
0
0
0

Apr. 01, 2002
P7BRQ41

80
80
0
0
0

May 13, 2002
May 13, 2002
P7BRQ57

0

May 27, 2002
P7BRQ63

0

Controls

>2560

(P7BRQ17)

320

(hexavalent)

160

1280

(P7BRQ16)

320

2560

(LeYM12)

20

160

Mono Ab (S193)

1280

(GB81)

0

Mono Ab (VK9)

0

(P7BRQ17)

(slovin lab wk 7)

Patient
Jan. 14, 2002
Jan. 14, 2002
P7BRQ2
0
0
0
0
0
40
0

4
Jan. 21, 2002
Jan. 21, 2002
P7BRQ6
0
0
0
0
0
20
20

Jan. 28, 2002
Jan. 28, 2002
P7BRQ10
0
0
0
80
0
40
0

Feb. 11, 2002
P7BRQ16
0
0
640
320
0
1280
0

Feb. 25, 2002
Feb. 25, 2002
P7BRQ26
0
0
160
40
0
320
0

Mar. 11, 2002
P7BRQ34
0
0
160
20
0
640
80

did not

Apr. 08, 2002

come in

Apr. 15, 2002
P7BRQ47

320
80
0
320
0

May 20, 2002
May 20, 2002
P7BRQ58

0

Jun. 03, 2002
P7BRQ66

80

Controls

>2560

(P7BRQ17)

320

(hexavalent)

320

>2560

(P7BRQ16)

160

>2560

(LeYM12)

20

160

Mono Ab (S193)

1280

(GB81)

20

Mono Ab (VK9)

0

(P7BRQ17)

(slovin lab wk 7)

Patient
Feb. 06, 2002
Feb. 06, 2002
P7BRQ15
0
0
0
0
0
0
0

5
Feb. 13, 2002
Feb. 13, 2002
P7BRQ22
0
0
0
20
0
0
0

Feb. 20, 2002
Feb. 20, 2002
P7BRQ25
0
0
0
0
0
0
0

Mar. 06, 2002
P7BRQ33
0
0
40
40
0
0
0

Mar. 20, 2002
Mar. 20, 2002
P7BRQ38
0
0
20
40
0
0
0

Apr. 03, 2002
P7BRQ42

160
40
0
0
0

May 01, 2002
P7BRQ51

0

Jun. 12, 2002
Jun. 12, 2002
P7BRQ71

Jun. 26, 2002

Controls

>2560

(P7BRQ17)

320

80

160

(hexavalent)

640

320

(P7BRQ16)

20

160

(LeYM12)

1280

Mono Ab (S193)

0

(GB81)

0

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

Patient
Feb. 06, 2002
Feb. 06, 2002
P7BRQ14
0
20
0
0
20
0
0

6
Feb. 13, 2002
Feb. 13, 2002
P7BRQ18
0
20
0
0
0
0
0

Feb. 20, 2002
Feb. 20, 2002
P7BRQ24
0
40
0
80
0
0
0

Mar. 06, 2002
P7BRQ31
0
20
320
320
0
0
0

Mar. 20, 2002
Mar. 20, 2002
P7BRQ39
0
20
160
320
0
0
0

Apr. 03, 2002
P7BRQ43

320
40
0
0
0

May 01, 2002
P7BRQ52

0

Jun. 12, 2002
Jun. 12, 2002
P7BRQ70

Jun. 26, 2002

Controls

>2560

320

(P7BRQ17)

80

640

(hexavalent)

640

320

(P7BRQ16)

0

80/160

(LeYM12)

1280

Mono Ab (S193)

0

(GB81)

0

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

ELISA Globo H
ELISA Tf(3
ELISA dOSM
ELISA

Ceramide(10
mcg)(May
for Tn (3 mcg)
sTn

Vaccine
Sample

mcg) (May 2002)
2002)
(June 2002)
(3 mcg)

Patient #
Date
Date
Serology Top
IgM
IgG
IgM
IgG
IgM
IgG
IgM

Patient
Jan. 16, 2002
Jan. 16, 2002
P7BRQ4
0
0
20

1
Jan. 23, 2002
Jan. 23, 2002
P7BRQ9
0
0
40

Jan. 30, 2002
Jan. 30, 2002
P7BRQ11
20
0
40

Feb. 13, 2002
P7BRQ19
20
320
640

Feb. 27, 2002
Feb. 27, 2002
P7BRQ28
0
80
1280

Mar. 13, 2002
P7BRQ37
20
160
1280

Apr. 10, 2002
P7BRQ44
20
80
1280

May 22, 2002
May 22, 2002
P7BRQ62

40
640

Jun. 05, 2002
P7BRQ67

Controls

(M62)

(MCG170)

(LeYM12)

Mono Ab (S193)

(GB81)

320

Mono Ab (VK9)

(P7BRQ17)

320

>2560

(slovin lab wk 7)

Patient
Jan. 16, 2002
Jan. 16, 2002
P7BRQ5
20
20

2
Jan. 23, 2002
Jan. 23, 2002
P7BRQ8
40
0
40

Jan. 30, 2002
Jan. 30, 2002
P7BRQ12
2560
160
640

Feb. 13, 2002
P7BRQ20
640
160
1280

Feb. 27, 2002
Feb. 27, 2002
P7BRQ27
640
160
1280

Mar. 13, 2002
P7BRQ36
320
320
640

Apr. 10, 2002
P7BRQ46
80
160
640

May 22, 2002
May 22, 2002
P7BRQ61

160
640

Jun. 05, 2002
P7BRQ68

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

320

Mono Ab (VK9)

(P7BRQ17)

320

>2560

(slovin lab wk 7)

Patient
Jan. 07, 2002
Jan. 07, 2002
P7BRQ1
0
0
0

3
Jan. 14, 2002
Jan. 14, 2002
P7BRQ3
0
0
0

Jan. 21, 2002
Jan. 21, 2002
P7BRQ7
320
0
80

Feb. 04, 2002
P7BRQ17
640
320
2560

Feb. 18, 2002
Feb. 18, 2002
P7BRQ23
320
320
1280

Mar. 04, 2002
P7BRQ30
320
1280
640

Apr. 01, 2002
P7BRQ41
80
320
320

May 13, 2002
May 13, 2002
P7BRQ57
20
160
320

May 27, 2002
P7BRQ63
20

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

320/640

Mono Ab (VK9)

1280/2560

(P7BRQ17)

320

2560

(slovin lab wk 7)

Patient
Jan. 14, 2002
Jan. 14, 2002
P7BRQ2
20
0
40

4
Jan. 21, 2002
Jan. 21, 2002
P7BRQ6
80
0
20

Jan. 28, 2002
Jan. 28, 2002
P7BRQ10
320
20
160

Feb. 11, 2002
P7BRQ16
640/1280
40
320

Feb. 25, 2002
Feb. 25, 2002
P7BRQ26
320
40
640

Mar. 11, 2002
P7BRQ34
320
160
160

did not

Apr. 08, 2002

come in

Apr. 15, 2002
P7BRQ47
160
160
160

May 20, 2002
May 20, 2002
P7BRQ58
40
320
160

Jun. 03, 2002
P7BRQ66
40

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

320/640

Mono Ab (VK9)

1280/2560

(P7BRQ17)

320

>2560

(slovin lab wk 7)

Patient
Feb. 06, 2002
Feb. 06, 2002
P7BRQ15
0
0
0

5
Feb. 13, 2002
Feb. 13, 2002
P7BRQ22
0
0
0

Feb. 20, 2002
Feb. 20, 2002
P7BRQ25
0
0
0

Mar. 06, 2002
P7BRQ33
20
20
40

Mar. 20, 2002
Mar. 20, 2002
P7BRQ38
0
0
40

Apr. 03, 2002
P7BRQ42
0
40
40

May 01, 2002
P7BRQ51
20
20
20

Jun. 12, 2002
Jun. 12, 2002
P7BRQ71

Jun. 26, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

320/640

(GB81)

1280/2560

Mono Ab (VK9)

320

>2560

(P7BRQ17)

320

1280

(slovin lab wk 7)

Patient
Feb. 06, 2002
Feb. 06, 2002
P7BRQ14
0
0
0

6
Feb. 13, 2002
Feb. 13, 2002
P7BRQ18
0
0
0

Feb. 20, 2002
Feb. 20, 2002
P7BRQ24
160
160
80

Mar. 06, 2002
P7BRQ31
160
160
320

Mar. 20, 2002
Mar. 20, 2002
P7BRQ39
80
40
160

Apr. 03, 2002
P7BRQ43
40
160
160

May 01, 2002
P7BRQ52
40
320
320

Jun. 12, 2002
Jun. 12, 2002
P7BRQ70

Jun. 26, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

320/640

(GB81)

1280/2560

Mono Ab (VK9)

320

2550

(P7BRQ17)

320

1280

(slovin lab wk 7)

ELISA GM2
ELISA MUC-1-1
ELISA LeY Ceramide
ELISA Globo H

(10 mcg)
5G (3
(10 mcg)
Ceramide(10

Patient
Vaccine
Sample

(April 2002)
mcg)(April 2002)
(April 2002)
mcg) (May 2002)

Name
Date
Date
Serology Top
IgG
IgM
IgG
IgM
IgG
IgM
IgG

Patient
Feb. 27, 2002
Feb. 27, 2002
P7BRQ29
0
0
0
0
0
0
0

7
Mar. 06, 2002
Mar. 06, 2002
P7BRQ32
0
0
0
0
0
0
0

Mar. 13, 2002
Mar. 13, 2002
P7BRQ35
0
20
20
320
0
0
0

Mar. 27, 2002
P7BRQ40
0
40
320
320
0
0
0

Apr. 10, 2002
Apr. 10, 2002
P7BRQ45
0
80
320
640
0
0
0

Apr. 24, 2002
P7BRQ49
0
80
160
320
0
0
0

May 22, 2002
P7BRQ60

0

Jul. 03, 2002
Jul. 03, 2002

Controls

>2560

(P7BRQ17)

320

80

640

(hexavalent)

640

320

0

1280

(P7BRQ16)

0

160

(LeYM12)

1280

Mono Ab (S193)

20

(GB81)

0

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

(June 2002)

(June 2002)

(July 2002)

(July 2002)

Patient
Apr. 22, 2002
Apr. 22, 2002
P7BRQ48

8
Apr. 29, 2002
Apr. 29, 2002
P7BRQ53

May 06, 2002
May 06, 2002
P7BRQ54

May 20, 2002
P7BRQ59

Jun. 03, 2002
Jun. 03, 2002
P7BRQ65

Jun. 17, 2002
P7BRQ72

Jul. 15, 2002

Aug. 26, 2002
Aug. 26, 2002

Sep. 09, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

Patient
Apr. 29, 2002
Apr. 29, 2002
P7BRQ50

9
May 06, 2002
May 06, 2002
P7BRQ55

May 13, 2002
May 13, 2002
P7BRQ56

May 27, 2002
P7BRQ64

Aug. 10, 2002
Jun. 10, 2002
P7BRQ69

Jun. 24, 2002

Jul. 22, 2002

Sep. 02, 2002
Sep. 02, 2002

Sep. 16, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

ELISA Globo H
ELISA Tf (10
ELISA dOSM for
ELISA

Ceramide(10
mcg)(May
Tn (3 mcg)
sTn

Patient
Vaccine
Sample

mcg) (May 2002)
2002)
(June 2002)
(3 mcg)

Name
Date
Date
Serology Top
IgM
IgG
IgM
IgG
IgM
IgG
IgM

Patient
Feb. 27, 2002
Feb. 27, 2002
P7BRQ29
0
0
20

7
Mar. 06, 2002
Mar. 06, 2002
P7BRQ32
0
0
0

Mar. 13, 2002
Mar. 13, 2002
P7BRQ35
0
320
160

Mar. 27, 2002
P7BRQ40
0
640/1280
160

Apr. 10, 2002
Apr. 10, 2002
P7BRQ45
0
640
80

Apr. 24, 2002
P7BRQ49
0
1280
80

May 22, 2002
P7BRQ60
0
640
80

Jul. 03, 2002
Jul. 03, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

320

(GB81)

1280/2560

Mono Ab (VK9)

640

2560

(P7BRQ17)

640

1280

(slovin lab wk 7)

Patient
Apr. 22, 2002
Apr. 22, 2002
P7BRQ48

8
Apr. 29, 2002
Apr. 29, 2002
P7BRQ53

May 06, 2002
May 06, 2002
P7BRQ54

May 20, 2002
P7BRQ59

Jun. 03, 2002
Jun. 03, 2002
P7BRQ65

Jun. 17, 2002
P7BRQ72

Jul. 15, 2002

Aug. 26, 2002
Aug. 26, 2002

Sep. 09, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

Patient
Apr. 29, 2002
Apr. 29, 2002
P7BRQ50

9
May 06, 2002
May 06, 2002
P7BRQ55

May 13, 2002
May 13, 2002
P7BRQ56

May 27, 2002
P7BRQ64

Aug. 10, 2002
Jun. 10, 2002
P7BRQ69

Jun. 24, 2002

Jul. 22, 2002

Sep. 02, 2002
Sep. 02, 2002

Sep. 16, 2002

Controls

(P7BRQ17)

(hexavalent)

(P7BRQ16)

(LeYM12)

Mono Ab (S193)

(GB81)

Mono Ab (VK9)

(P7BRQ17)

(slovin lab wk 7)

Notes

Monoclonals:

Dilutions VK9 1:200; S193 1:400

DOSM

Tested positive by ELISA with Monoclonals 5F4 and HB-TN1.

OSM

Tested positive by ELISA with Monoclonals 5F4, B72.3, and HB-TN1.

Shaded region denotes Pre sera (week 1)

All samples were tested in duplicate.

for patients Lewis and Smith, Lewis Y plates were coated at 0.3, future plates will be coated at 0.2.

Italics controls previously tested as positive.

Hexavalent Pilot study, protocol number #00-64, ELISA tested against TF(c)-HSA

Vaccination

1
2
3
4

5

Ag
Patient
Ab
wkl
2
3
7
12
19
21
31
33

TFc
1
Igm
40
40
40
40
>1280
40
40
40
40

HSA

IgG
20
20
>1280
320
80
80
80
160
320

2
IgM
NMA
80
160
160
80
40
40
20
20

IgG
10
NMA
10
40
80
NMA
NMA
20
40

3
Igm

40

IgG

NMA

4
IgM
40
20
320
80
80
80
NMA

IgG
NMA
NMA
640
80
40
160
320

5
IgM
NMA
20
160
20

IgG
10
NMA
10
20

6
IgM

40
640
640
640
160
80
80
160

IgG

640
>1280
>1280
>1280
>1280
>1280
>1280
>1280

7
IgM
NMA
40
80
640
160
80
40
80
80

IgG
10
320
NMA
NMA
40
20
80
20
80

8
IgM
NMA
NMA
160
160

IgG
NMA
NMA
10
80

9
IgM
NMA
NMA
NMA
20
NMA
NMA
NMA
NMA

IgG
NMA
NMA
40
NMA
640
80
>1280
160

10
IgM
NMA
10
160
160

IgG
NMA
NMA
40
20

11
IgM

20

IgG

NMA

12
Igm
10
40
160
>1280
80
640
80
20
160

IgG
NMA
NMA
NMA
NMA
>640
20
40
40
80

13
IgM

NMA

IgG

NMA

14
IgM
20
80
40
80
80
40
40
160
160

IgG
NMA
40
160
>1280
640
80
80
80
160

15
IgM
NMA
NMA
20
80
40
40

IgG
NMA
NMA
10
40
40
40

16
IgM
20
80
>1280

IgG
10
10
80

17
IgM
NMA
10
NMA
40
40
40
40
40
160

IgG
NMA
NMA

40
40
80
40
20
40

18
IgM
40
20
80
640
40
80
80
20
80

IgG
NMA
NMA
NMA
40
160
40
640
40
40

Positive Controls: IgM(19) 1:1280

IgG (7) 1:640

(−) Human AB Serum

As from Oct. 19, 2001 end pt. Titers:

(+) IgM: 640

IgG: 640

(−) IgM: NMA

IgG: NMA

Hexavalent Pilot study, protocol # 00-64 ELISA against glycosylated MUC1-1 (5 sites)

Vaccination

1
2
3
4

5

Ag
Patient
Number
Ab
wkl
2
3
7
12
19
21
31

MUC

1
Igm
NMA
40
>1280
>1280
>1280
>1280
>1280
>1280

1-1G5

IgG
NMA
NMA
80
160
>1280
640
>1280
>1280

32mer

2
IgM
NMA
NMA

640
10
NMA
10
20

IgG
NMA
NMA
10
40
40
20.00
40
160

3
Igm

20
640

IgG

NMA
40

4
Igm
NMA
NMA
320.00
>1280
>1280
>1280
640
640

IgG
NMA
NMA
10
320
160
>1280
>1280
>1280

5
IgM
10
40
>1280

>1280

IgG
NMA
NMA
160

>1280

6
IgM

NMA
320
>1280
320
320
160
80

IgG

NMA
160
>1280
320
160
160
160

7
IgM
NMA
NMA
40
640
640
80
80
40

IgG
NMA
NMA
640
>1280
>1280
>1280
>1280
>1280

8
IgM
NMA
NMA
160

IgG
NMA
NMA
10

9
IgM
NMA
NMA
40
160
80
20
20
10

IgG
NMA
NMA
NMA
40
20
10
80
40

10
Igm
NMA
NMA

IgG
NMA
NMA

11
IgM
NMA
NMA
10
40
20
160
160
80

IgG
NMA
NMA
10
320
160
40
40
20

12
Igm
40
40

IgG
NMA
NMA

13
Igm
NMA
NMA
20
80
80
320
320
160

IgG
NMA
NMA
20
20
40
320
320
160

14
Igm
80
20
160
160
40
40

IgG
NMA
NMA
NMA
NMA
40
20

15
Igm
NMA
NMA
640
640
640
10
10
10

IgG
NMA
NMA
640
640
640
160
80
80

16
Igm
NMA
20

IgG
NMA
20

17
IgM
NMA
20
320
160
40
640
320
80

IgG
NMA
NMA
10
80
640
40
640
160

Positive Controls: (7) IgM 1:2560

IgG 1:2560 Oct. 22, 2001

(−) AB Sera

Controls as of Oct. 15, 2001: (+) Igm: >1280

IgG: >1280

(−) IgM: NMA

IgG: NMA

Fourth Series of Experiments
Polyvalent Conjugate Vaccine for Cancer

Preliminary Data of Vaccination of High Risk Breast Cancer (BC) Patients (Pts) with a Heptavalent Antigen—Keyhole Limpet Hemocyanin (KLH) Conjugate Plus the Immunologic Adjuvant QS-21.

We have previously shown that following vaccination with single antigen (Ag)—KLH conjugates plus QS-21, the majority of BC pts generate specific antibody (AB) titers. (Clin Ca Res 6:1693, 2000; PNAS 98(6):3270, 2001; Proc ASCO 16:439a, 1997, 18:439a, 1999, 20:271a, 2001) Single Ag's tested have included MUC-1 (various peptide lengths), sTn clustered (c), GloboH and GM2. In an effort to improve and broaden the immune response, we treated BC pts with seven Ag's: 10 mcg each of GM2, GloboH, Lewisy; and 3 mcg each of TF(c), sTn(c), Tn(c) and glycosylated MUC-1, (32 amino acid (aa) sequence, glycosylated at 5 sites per 20 aa tandem repeat). Each Ag was conjugated to KLH and mixed with 100 mcg of QS-21. Heptavalent vaccines were administered subcutaneously during weeks 1, 2, 3, 7, and 19. We treated ten patients: median age 48 years (range 43-63 yrs); Stage IV=3, Stage 2 with 4 positive nodes=7. Nine pts have completed immunization. Toxicity was limited to transient grade 2 local skin reactions and grade 1-2 flu-like symptoms. IgM and IgG AB titers were considered positive for each antigen if there was at least an eightfold increase above baseline more than once, during weeks 1-19. Antibody responses are tabulated. (table) MUC1 and TF(c) seem most immunogenic. Flow cytometric analysis (FACS) was obtained pre and post therapy to detect binding of IgM and IgG AB against MCF-7 tumor cells. A positive FACS was defined as at least a threefold increase above baseline and was observed in 6/9 patients for IgM and 0/9 for IgG. Further analyses are ongoing. Our next cohort will evaluate the same antigens conjugated to KLH but with GP-100 as the immunologic adjuvant.

Number of pts with positive AB response/Number of pts evaluable

Ag
GM2
Ley
MUC1
TF(c)
sTn(c)
Tn(c)
GloboH

IgM
2/9
1/9
8/9
8/9
4/9
7/9
6/9

IgG
0/9
1/9
8/9
8/9
1/9
0/9
0/9

Objectives

- Determine immune response against seven antigens and cell lines expressing these antigens
- Evaluate toxicity

Background

- Preclinical data demonstrates that conjugation of an antigen with keyhole limpet hemocyanin (KLH) and addition of the immune adjuvant QS-21 augments immunogenicity (Cancer Immunol Immunother 41:185, 1985; Cancer Res 56:3315, 1996)
- Following vaccination with single antigen—KLH conjugates plus QS-21, most breast cancer patients generated IgM and IgG antibodies against the immunizing antigens (Clin Ca Res 6:1693, 2000; PNAS 98(6):3270, 2001; Proc ASCO 16:439a, 1997, 18:439a. 1999, 20:271a, 2001)
- These single antigens have included MUC-1 (various peptide lengths), sTn clustered (c), GloboH and GM2
- To broaden the immune response, seven antigens were individually conjugated to KLH and mixed with QS-21 to construct this heptavalent vaccine

Vaccine Components

- Antigens
  - Protein: glycosylated MUC-1 (32aa peptide)
  - Gangliosides: GM2, GloboH
  - Carbohydrates: LewisY, sTn(c), Tn(c),TF(c)
- Immunogenic protein carrier
  - KLH (by the following methods of conjugation):
    - MBS (m-maleimidobenzoyl-N-hydroxysuccinimide ester) linker for TF(c), sTn(c), Tn(c), and MUC-1
    - MMCCH (4-[4-N-maleimidomethyl] cyclohexane-1-carboxyl hydrazide) linker for GloboH and Le^Y
    - Direct reductive amination for GM2
- Immunologic Adjuvant
  - QS-21 (purified saponin fraction of tree bark)

Vaccine Components

Doses

Antigens*

GM2
10
mcg

MUC-1
3
mcg

LewisY
10
mcg

GloboH
10
mcg

TF(c)
3
mcg

Tn(c)
3
mcg

sTn (c)
3
mcg

Adjuvant

QS-21
100
mcg

*(each conjugated to KLH)

Treatment and Evaluation Plan

WEEK #

1
2
3
5
7
9
13
19
21
(q 3 months)

VACCINE
1
2
3

4

5

Blood
✓
✓
✓
✓
✓
✓
✓
✓
✓
✓

Samples

for

Immune

Response

Eligibility Criteria

Breast cancer patients with any one of the following features:

- Stage 1V (stable on hormone therapy [tx])
- Stage 1V (no evidence of disease [NED])
- Stage III
- Stage II (≧4 positive nodes)
- Ipsilateral breast or axillary recurrence
- Rising CA15-3 or CEA levels and NED

Patient Characteristics

- Total number of patients treated: 10
- Total number of vaccinations completed: 50
- *(One patient was delayed for unrelated issues)
- Median age: 48 years (range 43-63 years)
- Stage

II (with ≧4+ nodes):
7

IV (NED):
2

IV (stable on hormone tx):
1

n = 10

Common Toxicities

- Grade 1-2 injection site skin reactions
- Grade 1-2-flu-like symptoms
- No significant laboratory abnormalities
- No definite autoimmune reactions

Response Criteria: ELISA

- Serologic Response by ELISA (Enzyme-Linked Immunosorbent Assay)
  - IgM and IgG antibody titers were considered positive for each antigen if there was a eightfold increase above baseline more than once, during weeks 1-19
- Immunologic Response
- Patient was considered a responder if there was a serologic response to at least 3 of the 7 antigens Response Criteria: FACS and CDC
- Response by FACS (fluorescence activated cell sorter) was considered positive if there was the following increase above baseline:
  - ≧3-fold increase in percent gated positivity, AND
  - ≧1.5-fold increase on MFI (mean fluorescence intensity)
- Response by CDC (complement-dependent cytotoxicity) was considered positive if there was a 20% increase above baseline

Immune Response Data ELISA

GM2
MUC-1
Lewisy
GLOBOH
TF
Tn
sTn

IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG
IgM
IgG

1
−
−
+
+
−
−
−
−
+
+
−
−
−
−

2
+
−
+
+
−
−
+
−
+
+
+
−
+
−

3
+
−
+
+
−
−
+
−
+
+
+
−
+
−

4
−
−
+
+
+
−
+
+
+
+
+
−
−
−

5
−
−
−
+
−
−
−
−
−
−
−
−
−
−

6
−
−
+
+
−
−
+
−
+
+
+
−
+
−

7
+
−
+
+
−
−
−
−
+
+
+
−
−
−

8
−
−
+
+
−
−
+
−
+
+
−
−
+
−

9
−
−
+
+
−
−
+
−
+
+
−
−
−
+

10
−
−
+
+
−
−
+
−
+
+
−
−
+
−

·SUM
3
0
9
10
1
0
7
1
9
9
5
0
5
1

Immune Response Data FACS and CDC

FACS (IgM)
CDC

Patient
MCF-7
LSC
Du-175
MCF-7
LSC

1
+
+
+
−
−

2
−
+
−
+
+

3
+
−
−
−
−

4
+
+
+
+
+

5
−
−
−
−
−

6
+
+
−
+
−

7
+
+
−
−
+

8
−
+
−
+
−

9
+
+
+
−
−

10
−
−
−
+
−

• SUM
6
7
3
5
3

CONCLUSION

- Vaccination with a heptavalent antigen-KLH conjugate plus QS-21 is well tolerated in breast cancer patients
- IgM and IgG antibody responses (to at least 3 of 7 antigens) were observed in 8 patients and 2 patients respectively
- MUC1 and TF(c) to be appear the most immunogenic of the seven antigens in this vaccine
- IgM antibody binding to tumor cells (MCF-7, LSC, Du-145) by FACS analysis was observed in 6 patients, 7 patients, and 3 patients respectively
- There was no consistent evidence of IgG antibody binding to tumor cells by FACS
- There was evidence of CDC with the MCF-7 and LSC tumor cell lines in 5 patients and 3 patients respectively
- Our next cohort will evaluate the same antigens conjugated to KLH but with GP-100 as the immunologic adjuvant

	Number	Date	Country
	60303494	Jul 2001	US
	60347231	Jan 2002	US

	Number	Date	Country
Parent	12262729	Oct 2008	US
Child	13314521		US
Parent	10752945	Jan 2004	US
Child	12262729		US

	Number	Date	Country
Parent	PCT/US02/21348	Jul 2002	US
Child	10752945		US

POLYVALENT CONJUGATE VACCINE FOR CANCER

Information

Publication Number

Date Filed

Date Published

Inventors

Original Assignees

CPC

US Classifications

International Classifications

Abstract

Description

Claims

Parent Case Info

Government Interests

Provisional Applications (2)

Continuations (2)

Continuation in Parts (1)