TREA

METHODS FOR DIAGNOSING AND TREATING CANCER

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Information

  • Patent Application
  • 20180267046
  • Publication Number
    20180267046
  • Date Filed
    March 13, 2018
    6 years ago
  • Date Published
    September 20, 2018
    6 years ago
Information
Abstract
Disclosed is a method for identifying a subject at risk of developing a recurrent or metastatic cancer, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject. Also disclosed is method for treating a cancer comprising identifying a subject having one ore more PD-L1+ circulating tumor cells by detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, and administering a treatment to the subject.
Description
FIELD OF THE INVENTION

The present invention pertains to methods for diagnosing and treating cancer.


BACKGROUND OF THE INVENTION

Circulating tumor cells (CTCs) presence in circulation play active roles in mediating metastasis[1]. Enumeration of CTCs was reported as a prognostic predictor for metastatic colorectal cancer (mCRC) patients [2]. In most of the previous studies, the number of CTCs was enumerated from blood drawn by venipuncture of the forearm [3, 4]. It was suggested that the presence of circulating tumor cells expressing PD-L1 in non-small cell lung cancer patients at 6 months after the treatment of Nivolumab (PD-1 inhibitor) corresponds to a therapy escape or poor prognosis [5].


Until now, there is no promising method or kit for early detection or diagnosis of a metastatic cancer.


BRIEF SUMMARY OF THE INVENTION

The present invention is based on the unexpected finding that in patients having a gastrointestinal cancer or head and neck squamous-cell carcinoma, the presence/level of circulating tumor cells expressing PD-L1 (called as “PD-L1+ circulating tumor cells”) before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma, correlates with the metastasis of cancers or the prognosis of patients.


Accordingly, in one aspect, the present invention provides a method for identifying a subject at risk of developing a recurrent or metastatic cancer, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the presence of one or more PD-L1+ circulating tumor cells indicates that the subject is at risk of developing a recurrent or metastatic cancer, and wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.


In one embodiment of the present invention, the cancer is a gastrointestinal cancer, particularly a colorectal cancer. In another embodiment, the cancer is head and neck squamous-cell carcinoma.


In another aspect, the present invention provides a method for treating a cancer comprising: (a) identifying a subject having one or more PD-L1+ circulating tumor cells by detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma, and (b) administering a treatment to the subject.


In a further aspect, present invention provides a method for predicting prognosis of a patient having gastrointestinal cancer or head and neck squamous-cell carcinoma, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the patient, wherein the presence of one or more PD-L1+ circulating tumor cells indicates poor prognosis or overall survival of the patient, wherein the blood sample, the tissue fluid sample or the specimen is derived from the patient before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.


According to certain preferred embodiments of the present invention, said treatment is an immunotherapy. In some other embodiments, the subject is administered with an immunotherapy, in combination with a chemotherapy or a targeted therapy.


According to certain embodiments of the present invention, the cancer is a recurrent or metastatic cancer.


In one embodiment of the present invention, the cancer is a gastrointestinal cancer, particularly a colorectal cancer. In another embodiment, the cancer is head and neck squamous-cell carcinoma.


It is to be understood that both the foregoing general description and the following detailed description are exemplary and explanatory only and are not restrictive of the invention.





BRIEF DESCRIPTION OF THE SEVERAL VIEWS OF THE DRAWINGS

The foregoing summary, as well as the following detailed description of the invention, will be better understood when read in conjunction with the appended drawings. For the purpose of illustrating the invention, there are shown in the drawings embodiments which are presently preferred.


The patent or application file contains at least one color drawing. Copies of this patent or patent application publication with color drawing will be provided by the USPTO upon request and payment of the necessary fee.


In the drawings:



FIG. 1 illustrates the sample preparation for circulating tumor cell (CTC) enumeration via MiSelect R System.



FIG. 2 shows typical CTC images.



FIG. 3 shows the comparison of CTC counts in peripheral blood (PB) and mesenteric venous blood (MVB).



FIG. 4A shows the results on CTC counts in PB of colorectal cancer (CRC) patients at various stages. FIG. 4B shows the results on CTC counts in MVB of CRC patients at various stages.



FIG. 5 shows the heterogeneity of PD-L1 expressions on CTC.



FIG. 6 shows PD-L1+ CTC counts in PB and MVB.



FIG. 7 shows PD-L1+ CTC counts in MVB at various stages.



FIG. 8 shows the frequency of occurrence of PD-L1+ CTC at various stages.



FIG. 9 shows the heterogeneity of PD-L1 expressions on CTC





DETAILED DESCRIPTION OF THE INVENTION

In one aspect, the present invention provides a method for identifying a subject at risk of developing a recurrent or metastatic cancer, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the presence of PD-L1+ circulating tumor cells indicates that the subject is at risk of developing a recurrent or metastatic cancer, and wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.


According to the present invention, a higher level of the PD-L1+ circulating tumor cells indicates a higher risk of developing a recurrent or metastatic cancer.


In one embodiment of the present invention, the cancer is a gastrointestinal cancer, particularly a colorectal cancer. For gastrointestinal cancers, the blood sample is preferably a mesenteric venous blood sample. The mesenteric venous blood sample may be derived during surgeries of curative resection of the gastrointestinal cancer. The gastrointestinal cancer includes but is not limited an esophageal cancer, a gastric cancer, a gastrointestinal stromal tumor, a pancreatic cancer, a liver cancer, a gallbladder cancer, a colorectal cancer, and an anal cancer. In a particular example of the present invention, the cancer is a colorectal cancer.


In another embodiment, the cancer is head and neck squamous-cell carcinoma.


In another aspect, the present invention provides a method for treating a cancer comprising: (a) identifying a subject having PD-L1+ circulating tumor cells by detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma, and (b) administering a treatment to the subject.


In a further aspect, present invention provides a method for predicting prognosis of a patient having a gastrointestinal cancer or head and neck squamous-cell carcinoma, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the patient, wherein the presence of one or more PD-L1+ circulating tumor cells indicates poor prognosis or overall survival of the patient, and wherein the blood sample, the tissue fluid sample or the specimen is derived from the patient before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.


According to the present invention, a higher level of the PD-L1+ circulating tumor cells indicates a worse prognosis of the patient.


The treatment includes but is not limited to immunotherapy, chemotherapy, radiation therapy, hormone therapy, or a combination thereof.


According to certain preferred embodiments of the present invention, said treatment is an immunotherapy. In some other embodiments, the subject is administered with an immunotherapy, in combination with a chemotherapy or a targeted therapy.


According to certain embodiments of the present invention, the cancer is a recurrent or metastatic cancer.


In one embodiment of the present invention, the cancer is a gastrointestinal cancer, particularly a colorectal cancer. In another embodiment, the cancer is head and neck squamous-cell carcinoma.


For gastrointestinal cancers, the blood sample is preferably a mesenteric venous blood sample. The mesenteric venous blood sample may be derived during surgeries of curative resection of the gastrointestinal cancer.


In certain embodiments of the present invention, the cancer is a gastrointestinal cancer, which includes, but is not limited to, an esophageal cancer, a gastric cancer, a gastrointestinal stromal tumor, a pancreatic cancer, a liver cancer, a gallbladder cancer, a colorectal cancer, and an anal cancer. In a particular example of the present invention, the cancer is a colorectal cancer.


In some other embodiments of the present invention, the cancer is head and neck squamous-cell carcinoma.


The present invention is further illustrated by the following examples, which are provided for the purpose of demonstration rather than limitation.


Examples

Materials and Methods


1. Patient Characteristics


A total of 116 patients who underwent curative surgical resection at Taipei Veterans General Hospital between April 2016 and September 2017 were enrolled. A total 26 HNSCC, 9 HCC, 5 UC and 2 RCC patients who underwent receiving immunotherapy at Taipei Veterans General Hospital between October 2016 and September 2017 were also enrolled. The enrollment procedures followed the protocols approved by the Internal Review Board of Taipei Veterans General Hospital. All patients provided written informed consent. Patients who prior to colonoscopy examination or suspected of having colorectal cancer (CRC) with unconfirmed clinical stages were recruited. Six patients who had histological diagnosed tubular adenoma were also enrolled. The average (±SD) age of the assessable patients was 63.6±12.5 years (median, 64) (see Table 1 below). Primary tumor staging was confirmed by histologic examination of the resected primary tumor. Based on histologic examination, the subjects consisted of 116 CRC patients (24 stage I, 38 stage II, 42 stage III and 12 stage IV, respectively).









TABLE 1







Clinicopathological characteristics of the study population












Stage I
Stage II
Stage III
Stage IV



(n = 24)
(n = 38)
(n = 42)
(n = 12)















Age
64
68
64
59


Median (range)
(37-79)
(38-92)
(37-84)
(47-90)


Gender


Male
10
28
22
8


Female
14
10
20
4


Tumor location


Colon
20
27
29
9


Rectum
4
11
13
3


T stage


T1
14
0
3
0


T2
10
0
5
1


T3
0
24
21
4


T4
0
14
13
7


N stage


N0
24
38
0
2


N1
0
0
31
4


N2
0
0
11
6


CEA (≥5 ng/mL)
3
17
17
10


CA 19-9 (≥37 ng/mL)
1
7
8
5









2. Blood Sample Collection


Blood samples for CTC analysis were obtained from CRC patients before curative resection of tumor. Sampling of blood from the antecubital veins of patients with CRC was conducted before surgery. During surgery, mesenteric venous blood samples were drawn from the main drainage vein of the diseased segment of the colon, for example, the inferior mesenteric vein for cancer of the sigmoid colon or rectum or the ileocolic vein if the tumor was located on the right side of the colon. To minimize the possibility of releasing CTCs by mechanical manipulation, colonoscopy was scheduled at least 1 day before the surgery. The surgical approach sought vascular control first, that is, ligation of the feeding artery at the beginning, followed by mesenteric vein cannulation and blood drawing. The tumor was left untouched until late in the surgery. Peripheral blood (PB) and mesenteric venous blood (MVB) samples for CTC analysis were obtained from 116 patients. Blood samples for CTC analysis were also obtained from other cancer patients before drug administrations.


3. CTC Enumeration and PD-L1 Expression Test on CTC


The sample preparation is shown in FIG. 1. Transfer two 4-ml aliquots of blood from K2EDTA tube into two correspondingly labeled 50 ml conical centrifuge tubes. Samples incubate with Sorting Reagent (PE-conjugated anti-EpCAM antibody) of SelectKit for 20 minutes at room temperature. After staining, spilt each 4 ml blood to two 2-ml aliquots into two correspondingly labeled 50 ml conical centrifuge tubes, add 24 ml ISOTON Diluent into each tube. Centrifuge the sample at 800×g for a full 10 minutes with the brake off using a swing bucket centrifuge at room temperature. Following centrifugation, remove 24 ml supernatant of each tube and mix the samples following recovery of two 2-ml aliquots into 4 ml aliquots for CTC analysis. Process on the MiSelect R System within 1 hour of sample preparation.


MiSelect R System with SelectChip Dual (MiCareo Taiwan Co., Ltd) can sort and enrich CTC. Once the aliquots containing CTCs have been collected in SelectChip, blood cells, especially RBCs, are removed from the CTCs by an on-chip filtration system. After enrichment of CTCs, Fixation and Staining Reagent of SelectKit are automated added for identification and enumeration of CTCs. Anti-panCK APC is specific targeting for the intracellular protein cytokeratin, DAPI stains for the cell nucleus and anti-CD45 FITC is specific for leukocytes. An event is classified as a tumor cell when its morphological features are consistent with that of a tumor cell and it exhibits the phenotype EpCAM+, CK+, DAN+, and CD45.


The CTC number will be counted and analyzed by operators and recorded directly. For further immunostaining on CTCs, anti-PD-L1 will be automated injecting into SelectChip for labeling CTC on MiSelect R System. The fluorescence images of each biomarkers on CTC will be taken and intensity of the biomarkers will be recorded for further analysis.


4. Statistical Analyses


All data were statistically analyzed with SPSS software (v19.0) and GraphPad Prism (v5.0). The distributions of continuous variables were described as median values and ranges. The Mann-Whitney U test and the Wilcoxon-signed ranks test were performed to evaluate the differences between groups, as appropriate. All P-values were two-sided. P-values of less than 0.05 indicated statistical significance.


Results


1. Prevalence of CTC in PB and MVB


CTC was defined as a cell with intact nucleus, expressing EpCAM and cytokeratin, but absence of CD45 expression. Typical CTC images were demonstrated in FIG. 2. The EpCAM expression showed heterogeneity among CTCs even within the same CRC patient. CTCs were barely found in PB (mean, 0.17±0.89 per 8 ml of whole blood; range=0-8, n=116) but more abundant in MVB (mean, 7.1±48.1 per 8 ml of whole blood; range=0-515, n=116) (FIG. 3; P<0.001).


2. Distribution of CTC Counts and Detection Rates


The CTC counts for CRC patients are presented in Table 2 below and in FIG. 4. CTC count ranged from 0 to 8 in non-metastatic CRC and 0 to 4 in metastatic CRC in PB; In MVB, CTC count ranged from 0 to 515 in non-metastatic CRC and 0 to 20 in metastatic CRC. The overall detection rate of CTC is 6% and 40.5% in PB and MVB, respectively. Within each subgroup, the detection rate increased with the severity of the subgroup's condition. In MVB, CTC detection rate was 20.8%, 42.1%, 45.2% and 58.3% for stage I, II, III, and IV respectively. Besides, the amount of CTC was significantly more abundant in late stages than early stages (FIG. 4).









TABLE 2







CTC count in various stages of PB and MVB











No. of

Range of



cases

CTC number in



N = 116

8 ml


















Detection rate






in MVB %



Stage I
24
20.8% (5/24) 
0-9



Stage II
38
42.1% (16/38)
 0-20



Stage III
42
45.2% (19/42)
 0-515



Stage IV
12
58.3% (7/12) 
 0-20





P-value =





0.0298





Detection rate





in PB %



Stage I
24
4.2% (1/24)
0-1



Stage II
38
10.5% (4/38) 
0-8



Stage III
42
2.4% (1/42)
0-1



Stage IV
12
16.6% (2/12) 
0-4





P-value =





0.7053










3. Relationships Between CTC Number and Clinicopathological Characteristics


We explored the bivariate relationship between CTC numbers (present or absent) versus various clinical and pathological parameters. The results are shown in Table 3 below. The clinical staging (TNM) positively correlated to CTC number in MVB (Table 2) and pre-operative serum CEA level and tumor invasion depth (pT) positively correlated to CTC levels in MVB. No association was noted between CTC numbers and presence of liver or lung metastases, primary CRC differentiation, histology, nodal status (N), lymphatic/venous invasion/perineural invasion, inflammatory change around carcinoma, invasion pattern of cancer tissue and pre-operative serum CA-19-9 level.









TABLE 3







Correlation between clinicopathological parameter and


the present of CTCs










Clinicopathological





variables
CTC present %
CTC absent %
P value













T stage


0.018


T1/T2
17% (6/34)
83% (28/34)


T3/T4
48% (41/84)
52% (43/84)


N stage


0.13


N0
34% (22/65)
66% (43/65)


N1
49% (25/51)
51% (26/51)


CEA


0.049


 ≥5 mg/mL
53% (23/44)
47% (21/44)


  <5 mg/mL
33% (23/71)
67% (48/71)


CA-199


0.33


≥37 mg/mL
50% (11/22)
50% (11/22)


 <37 mg/mL
37% (35/94)
63% (49/94)









4. PD-L1 Biomarker Assessment on CTCs in CRC Patients


CTCs isolated from PB and MVB were examined for PD-L1 protein expression. The PD-L1 biomarker expression showed heterogeneity among isolated CTCs between patients and within the same blood sample (FIG. 5). PD-L1 status on CTC in PB was evaluated in 8 patients with detectable CTC (see Table 4 below). PD-L1 status on CTC in MVB was evaluated in 47 patients with detectable CTC. Among these 47 patients, 31 (65.9%) showed a subpopulation of PD-L1+ CTCs (see FIG. 6 and Table 5 below). The number of PD-L1+ CTCs varied from 1 to 33 (median=3) and the fraction of PD-L1+ CTCs ranged from 16 to 100% of the whole number of detectable CTCs. The PD-L1+ CTC number gradually increased with stages (FIG. 7) and the frequency of PD-L1+ CTCs among CTCs also increased with stages (FIG. 8).









TABLE 4







Number of PD-L1+ CTC in PB of various stages












Patients


PD-L1+CTC



number
Stage
CTC number
number







0031
I
1
0



0009
II
1
0



0078
II
1
0



0090
II
2
1



0113
II
3
0



0057
III
1
0



0004
IV
1
0



0075
IV
4
3

















TABLE 5







Number of PD-L1+ CTC in MVB of various stages












Patients


PD-L1+CTC



number
Stage
CTC number
number
















0011
I
1
0



0021
I
3
2



0031
I
1
0



0123
I
2
0



0129
I
9
1



0001
II
5
0



0009
II
2
2



0016
II
1
0



0037
II
2
1



0046
II
2
1



0051
II
2
0



0055
II
8
4



0060
II
1
0



0089
II
1
0



0091
II
1
0



0094
II
11
6



0096
II
2
0



0097
II
1
0



0103
II
15
8



0118
II
3
1



0139
II
20
14



0006
III
1
0



0012
III
4
4



0025
III
1
0



0030
III
1
1



0057
III
1
1



0069
III
5
5



0076
III
1
0



0077
III
3
3



0082
III
45
33



0084
III
21
12



0085
III
5
3



0086
III
2
1



0098
III
2
1



0100
III
1
1



0102
III
1
1



0104
III
2
1



0106
III
1
1



0134
III
1
0



0141
III
6
2



0004
IV
5
0



0017
IV
17
16



0028
IV
13
2



0034
IV
5
3



0038
IV
2
2



0068
IV
2
2



0075
IV
10
9










5. Relationships Between PD-L1+ CTC Number and Clinicopathological Characteristics in CRC Patients


We explored the bivariate relationship between PD-L1+ CTC numbers (present or absent) versus various clinical and pathological parameters. The results are shown in Table 6 and Table 7 below. The clinical staging (TNM) positively correlated to PD-L1+ CTC number in MVB (Table 6) and pre-operative serum CEA level, tumor invasion depth (pT), nodal status (N), positively correlated to PD-L1+ CTC levels in MVB. Besides, the primary CRC lymphatic and venous invasion were correlated to PD-L1+ CTC levels in MVB (Table 7). No association was noted between PD-L1+ CTC numbers and primary CRC differentiation, perineural invasion, inflammatory change around carcinoma, invasion pattern of cancer tissue and pre-operative serum CA-19-9 level.









TABLE 6







Correlation between PD-L1(+) CTC presence and clinical stage










Detection rate of
PD-L1(+) rate in



PD-L1(+) CTC
CTC detected patients



N = 116
N = 47















Stage I
 8.3% (2/24)
40.0% (2/5)



Stage II
21.1% (8/38)
 50.0% (8/16)



Stage III
 35.7% (15/42)
 78.9% (15/19)



Stage IV
50.0% (6/12)
85.7% (6/7)




P-value = 0.0017
P-value = 0.0178

















TABLE 7







Correlation between clinicopathological parameter and


the present of PD-L1+ CTCs











PD-L1(+)





CTC
PD-L1(+) CTC


Clinicopathological variables
present (%)
absent (%)
P value













T stage


0.016


T1/T2
6% (2/33)
94% (31/33)


T3/T4
48% (23/83)
52% (60/83)


N stage


0.013


N0
12% (8/65) 
88% (57/65)


N1
33% (17/51)
67% (34/51)


CEA


0.002


 ≥5 mg/mL
36% (17/47)
64% (30/47)


  <5 mg/mL
10% (7/67) 
90% (7/67) 


CA-199


0.13


≥37 mg/mL
33% (7/21) 
67% (14/21)


 <37 mg/mL
17% (16/92)
83% (76/92)


Blood Vascular Invasion


0.014


(+)
42% (11/26)
58% (15/26)


(−)
17% (14/84)
83% (70/84)


Lymphatic Vascular Invasion


0.0042


(+)
36% (11/30)
64% (19/30)


(−)
18% (14/80)
82% (66/80)









6. PD-L1 Biomarker Assessment on CTCs in Other Cancer Patients


The overall detection rate of CTC is 31%, 55% and 40% in patients with head and neck squamous-cell carcinoma (HNSCC), hepatocellular carcinoma (HCC) and uterine cancer (UC), respectively (see Table 8 below). CTCs isolated from HNSCC, HCC and UC patients were examined for PD-L1 protein expression. The PD-L1 biomarker expression showed heterogeneity among isolated CTCs between patients and within the same blood sample (FIG. 9). PD-L1 status on CTC was evaluated in patients with detectable CTCs. Among these patients, 100% of HNSCC, 50% of HCC and 100% of UC showed a subpopulation of PD-L1+ CTCs (Table 8). The presence of PD-L1(+) CTC significantly correlates with disease progression in HNSCC patients (see Table 9 below).









TABLE 8







CTC and PD-L1(+) CTC detection rate in advanced cancers













PD-L1 positive


Cancer
CTC
PD-L1(+) rate in CTC
rate in CTC


type
detection rate %
detected patients %
(Range)





HNSCC
 31% (8/26)
100% (8/8)
12.5-100%


N = 26


HCC
55% (4/9)
 50% (2/4)
  50-100%


N = 9


UC
40% (2/5)
100% (2/2)
100%


N = 5


RCC
0/2
0%
N.A.


N = 2
















TABLE 9







Correlation between CTC or PD-L1(+) CTC presence and


disease progression









CTC/PD-L1(+) CTC















P-



Clinical outcome
present
absent
value







Progression disease
7
4
0.034



Complete response/
0
6



Partial response/



Stable disease










REFERENCES



  • 1. Pantel, K., C. Alix-Panabieres, and S. Riethdorf, Nat Rev Clin Oncol, 2009. 6(6): p. 339-51.

  • 2. Cohen, S. J., et al., J Clin Oncol, 2008. 26(19): p. 3213-21.

  • 3. Thorsteinsson, M., G. Soletormos, and P. Jess, Anticancer Res, 2011. 31(2): p. 613-7.

  • 4. Sastre, J., et al., Ann Oncol, 2008. 19(5): p. 935-8.

  • 5. Nicolazzo, C. et al., Sci Rep 2016 Aug. 24; 6:31726.


Claims
  • 1. A method for identifying a subject at risk of developing a recurrent or metastatic cancer, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the presence of one or more PD-L1+ circulating tumor cells indicates that the subject is at risk of developing a recurrent or metastatic cancer, and wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.
  • 2. A method for treating a cancer comprising: identifying a subject having PD-L1+ circulating tumor cells by detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the subject, wherein the subject has a gastrointestinal cancer or head and neck squamous-cell carcinoma and the blood sample, the tissue fluid sample or the specimen is derived from the subject before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma; andadministering a treatment to the subject.
  • 3. The method of claim 2, wherein the cancer is a recurrent or metastatic cancer.
  • 4. The method of claim 2, wherein the treatment includes an immunotherapy.
  • 5. The method of claim 3, wherein the treatment includes an immunotherapy.
  • 6. The method of claim 1, wherein the cancer is a gastrointestinal cancer.
  • 7. The method of claim 2, wherein the cancer is a gastrointestinal cancer.
  • 8. The method of claim 6, wherein the gastrointestinal cancer is a colorectal cancer.
  • 9. The method of claim 7, wherein the gastrointestinal cancer is a colorectal cancer.
  • 10. The method of claim 6, wherein the blood sample is a mesenteric venous blood sample.
  • 11. The method of claim 7, wherein the blood sample is a mesenteric venous blood sample.
  • 12. A method for predicting prognosis of a patient having gastrointestinal cancer or head and neck squamous-cell carcinoma, comprising detecting PD-L1+ circulating tumor cells in a blood sample, a tissue fluid sample or a specimen of the patient, wherein the presence of one or more PD-L1+ circulating tumor cells indicates poor prognosis of the patient, and wherein the tissue fluid sample or the specimen is derived from the patient before a therapy for, or during a surgery of curative resection of the gastrointestinal cancer or head and neck squamous-cell carcinoma.
  • 13. The method of claim 12, wherein the patient has a gastrointestinal cancer.
  • 14. The method of claim 13, wherein the gastrointestinal cancer is a colorectal cancer.
  • 15. The method of claim 13, wherein the blood sample is a mesenteric venous blood sample.
CROSS REFERENCE TO RELATED APPLICATIONS

This non-provisional application claims the benefit under 35 U.S.C. § 119(e) to U.S. Provisional Application No. 62/471,083, filed on Mar. 14, 2017, and to U.S. Provisional Application No. 62/584,634, filed on Nov. 10, 2017, all of which are hereby expressly incorporated by reference into the present application.

Provisional Applications (2)
Number Date Country
62471083 Mar 2017 US
62584634 Nov 2017 US