Conventional cancer therapy is rarely curative and can have profound adverse side effects. In part, this stems from the cell cycle specific mechanism of action of most chemotherapeutic drugs, which renders them less effective against a population of cells representing all cell cycle phases.
The cell cycle is the series of events occurring in a cell leading to its division and duplication. In eukaryotic cells, the cycle can be divided into two periods, interphase and mitosis. Transit through these two periods of the cell cycle is known as progression or proliferation. During interphase, the cell grows, accumulates nutrients needed for mitosis and duplicates its DNA. During mitosis, the cell splits itself into two distinct daughter cells. Interphase includes three distinct phases, Gap 1 (G1) phase, S phase and Gap 2 (G2) phase while mitosis includes two processes. G1 phase includes the cell increasing in size, biosynthetic activities of the cell increasing and the synthesis of enzymes needed for DNA replication in the subsequent step. S phase includes the beginning of DNA synthesis and replication of all of the chromosomes. G2 phase lasts until the cell enters mitosis and includes protein synthesis including the production of microtubules for mitosis. Mitosis includes a process where the cell's chromosomes are divided between the two daughter cells and a cytokinesis process where the original cell's cytoplasm divides forming two distinct daughter cells. The cell cycle also includes a resting phase, typically referred to as G0. The boundaries between the various phases, for example the boundary between the G1 and S phase is referred to as a cell cycle checkpoint.
The progression of the cell cycle can be inhibited, so that a particular cell stops the cycle at a point, a cellular checkpoint, before proceeding to the next phase. Cell cycle checkpoints are located between the different phases of the cell cycle, with two of the checkpoints being at the interface between the G1 and the S phase (G1/S) and the interface between the G2 and M phase. A cell cycle inhibitor can stop the progression of a cell from passing to the next phase, for example a cell can be inhibited at the G1/S cell cycle checkpoint, which forces the cell to remain in the G1 phase until the inhibitor is removed.
In any particular cancer cell population or tumor in an individual, the length of the cell cycle is variable. This variability is due to differing periods spent in G1 of G0 while the length of time from the beginning of S phase to the end of M phase is relatively constant.
Conventional chemotherapeutic treatment only disrupts events in the S or M phase of the cell cycle, leaving cells in the other phases of the cell cycle relatively unharmed. For example, an alkylating agent will act in the S phase while microtubule stabilizing or disruption drugs act in the M phase. Unfortunately, a particular cell is not likely to be at the S or M phase of the cell cycle at a specific time. To compensate for this, chemotherapeutic drugs must be administered repetitively, over long periods of time to increase the chances of reaching a cell which is in the specific cell cycle phase. This repetitive administration translates into larger doses of harmful drugs and an increased toxicity in a subject.
What is desired is a treatment to arrest the cell cycle for a clinically relevant fraction of cells at the G1/S cell cycle checkpoint, so that the efficacy of chemotherapeutics can be enhanced.
The present invention provides a method for treating a disease or condition in a mammal which comprises the steps of; administering a therapeutically effective amount of a T type calcium channel inhibitor to effectively slow or stop progression of eukaryotic cells through the S, G2 and M phases of the cell cycle to increase the proportion of the eukaryotic cells in the G1 phase, stopping administration of the T type calcium channel inhibitor for a period of time, and administering a dosage selected from the group consisting of a dosage of at least one chemotherapeutic agent, a dosage of radiation, and combinations thereof, to kill the proportion of eukaryotic cells progressing past the G1 phase of the cell cycle after the stopping of the administration of the T type calcium channel inhibitor.
In describing and claiming the invention, the following terminology will be used in accordance with the definitions set forth below.
As used herein, the term “treating” includes administering therapy to prevent, cure, ameliorate, reduce, inhibit or alleviate/prevent the symptoms associated with, a specific disorder, disease, injury or condition. For example treating cancer includes inhibition or complete growth arrest of a tumor, reduction in the number of tumor cells, reduction in tumor size, inhibition of tumor cell infiltration into peripheral organs/tissues, inhibition of metastasis as well as relief, to some extent, of one or more symptoms associated with the disorder. The treatment of cancer also includes the administration of a therapeutic agent that directly decreases the pathology of tumor cells, or renders the tumor cells more susceptible to treatment by other therapeutic agents, e.g., radiation and/or chemotherapy. As used herein, the term “treating” includes prophylaxis of the specific disorder or condition, or alleviation of the symptoms associated with a specific disorder or condition and/or preventing or eliminating said symptoms.
As used herein, the term “pharmaceutically acceptable carrier, vehicle or diluent” includes any of the standard pharmaceutical carriers, such as a phosphate buffered saline solution, water, emulsions such as an oil/water or water/oil emulsion, and various types of wetting agents. The term also encompasses any of the agents approved by a regulatory agency of the US Federal government or listed in the US Pharmacopeia for use in animals, including humans.
The term “therapeutically effective amount” means an amount of a compound of the present invention that ameliorates, attenuates, reduces or eliminates a particular disease or condition or prevents or delays the onset of a particular disease or condition.
By “mammal” it is meant to refer to all mammals, including, for example, primates such as humans and monkeys. Examples of other mammals included herein are rabbits, dogs, cats, cattle, goats, sheep, mice, rats and horses. Preferably, the mammal is a female or male human.
The expression “pre-cancerous condition” refers to a growth that is not malignant but is likely to become so if not treated. A “pre-cancerous condition” is also known as “pre-malignant condition” by one of ordinary skill in the art.
It is understood to one skilled in the art that “T type calcium channel blockers” are also known as “T type calcium channel inhibitors”.
As used herein, the term “cell cycle inhibitor” refers to a compound which is capable of slowing or stopping progression of a cell or cells in one stage of the cell cycle from progressing to the subsequent stage of the cell cycle.
As used herein, the term “cytotoxin” refers to a compound which is capable of causing necrosis or apoptosis to a cell which is affected by the compound.
Varying lengths of the cell cycle are determined predominately by the time spent in the G1 phase. Because of this, any particular cell in a population will reside in G1 for a period of time before the cell enters the S phase of the cell cycle. To stop the cell cycle from continuing past a cell cycle checkpoint, a cell cycle inhibitor, including a T type calcium channel inhibitor can be administered.
The cell cycle inhibitor is first administered to a mammal in a therapeutically effective amount to effectively slow or stop progression of eukaryotic cells through the S, G2 and M phases of the cell cycle, thereby increasing the proportion of the eukaryotic cells at the cell cycle checkpoint between the G1 and S phase (G1/S). The mammal may be a human. This method may be used to treat cancer and pre-cancerous conditions, and cancerous and pre-cancerous tumors in a mammal.
The administration of the cell cycle inhibitor causes asynchronously progressing or proliferating cancer cells in a population to accumulate at G1/S as they proceed through the cell cycle because their ability to proceed to the S phase is arrested by the cell cycle inhibitor. For a cell to move from G1 phase to S phase through the cell cycle checkpoint, the cell requires influx of extracellular calcium to trigger biochemical cascades that are necessary for the progression. Removal of calcium from the extracellular medium blocks cell cycle transit for each cell. This blocking can be accomplished through administration of a T type calcium channel inhibitor. Suitable T type calcium channel inhibitors include mibefradil, efonidipine, ethosuxamide, sutinib, TTL-1177 (a proprietary compound, described in reference: Gray, L. S., Perez-Reyes, E., Gomora, J. C., Haverstick, D. M., Shattock, M., McLatchie, L., Harper, J., Brooks, G., Heady, T., and MacDonald, T. L. (2004) Cell Calcium 36, 489-497) and nickel, among others. Thus, each cell persists in G1 phase as long as it would in the presence of extracellular calcium, but becomes locked in place when G1/S is reached without calcium, thereby synchronizing cells at G1/S. Calcium influx to a cell is necessary for progression and transit through the cell cycle. This is further described in Example 1 below.
The administration of the cell cycle inhibitor increases the percentage of cells at G1/S. Subsequent to this administration, a dosage of at least one chemotherapeutic agent, a dosage of radiation, or a dosage of both are administered, the dosage being targeted to kill cells in the S phase of the cell cycle. The chemotherapeutic agent can be a cancer chemotherapeutic, a cytotoxin or combinations thereof. The cytotoxin can be an alkylating agent. The cancer chemotherapeutic can be an anti-metabolite or an anti-mitotic and can be selected from the following examples; temozolamide (Temp), 5-fluorouracil, 6-mecaptopurine, bleomycin, carboplatin, cisplatin, dacarbazine, doxorubicin, epirubicin, etoposide, hydroxyurea, ifosfamide, irinotecan, topotecan, metotrexate, mitoxantrone, oxaliplatin, paclitaxel, doocetaxol, vinblastine, vincristine, vinorelbine, vindesine, mitomycin C and combinations thereof. The dosage of at least one chemotherapeutic agent can be administered before, after or during a dosage of radiation. The dosage of radiation can be administered before, after or during a dosage of at least one chemotherapeutic. The period between the first administration of the cell cycle inhibitor and the cytotoxin, allows the accumulation of cells at G1/S of the cell cycle. This method increases the percentage of the cells which are in the S or M phase, thereby increasing the effectiveness of the dosage of at least one chemotherapeutic agent, the dosage of radiation, or the dosage of both and subsequently reducing the toxic load required to kill a predetermined amount of eukaryotic cells.
The cell cycle inhibitor can be administered a second time, after the administration of the dosage of at least one chemotherapeutic agent, the dosage of radiation, or the dosage of both to slow re-growth of targeted cells or tumors so that further administrations of the dosage can be provided as needed. This second administration of a cell cycle inhibitor will resynchronize a percentage of the population of cells at G1/S.
The cell cycle inhibitor can be administered through several routes including parenteral, intravenous, intramuscular, intraperitoneal, intrathecal, suppository, transdermal, topical, or oral. Oral administration of the cell cycle inhibitor is most preferred. An oral administration can be administered as a dosage unit, typically a pill or capsule along with a pharmaceutically acceptable carrier.
The T type calcium channel inhibitors restrict the influx of extracellular calcium into the cell which is critical for a number of vital cellular processes. The calcium necessary for these processes comes from the extracellular milieu via influx through calcium channels. Calcium channels are grouped into several families based upon sequence analysis, biophysical characteristics and pharmacological sensitivity. These calcium channels have been implicated in regulation of blood pressure, cardiac rhythm and cellular proliferation. Studies also suggest that T-type calcium channels may play an important role in age related macular degeneration. At least one pharmacological agent, mibefradil, has been proven to be clinically effective because of inhibition of T channel function. Inhibitors of calcium entry are useful for treating hypertension, cardiac arrhythmia and clinically deleterious cellular proliferation.
T type calcium channels are present in cells, cell lines and specifically cancer cell lines. Specifically, the Cav3.2 isoform of T type calcium channels has been shown to be aberrantly expressed in breast cancer tissue as compared to normal adjacent breast tissue in Japanese women, as discussed in reference Asaga, S., Ueda, M., Jinno, H., Kikuchi, K., Itano, O., Ikeda, T., and Kitajima, M. (2006) Anticancer Res 26, 35-42.
Cell cycle inhibitors effectively stop or slow progression of eukaryotic cells at cell cycle checkpoints, including G1/S, which is further explained in Example 2 below. Further, administration of cell cycle inhibitors effectively slows growth or proliferation of a disease or condition, as explained in Example 3 below.
Subsequent to administration of the cell cycle inhibitor, there is a period during which no cell cycle inhibitor is added. This period can range from about 0 hours to about 336 hours. This period allows the cells which have accumulated at G1/S to enter the S phase of the cell cycle. Through administration of the cell cycle inhibitor, about 5% to about 25% of cells will have accumulated at G1/S. The increase in number of cells in the S phase makes an administered dosage of at least one chemotherapeutic agent, dosage of radiation, or the dosage of both more effective because a large percentage of cells will be affected by each dose. By “affected” is meant killed or distilled.
Subsequent to the period where no cell cycle inhibitor is added, a dosage of at least one chemotherapeutic agent, a dosage of radiation, or a dosage of both is administered to kill a proportion of cells in the S. By “killed” is meant that the cell undergoes apoptosis or necrosis. The specific dosage of at least one chemotherapeutic agent, dosage of radiation, or dosage of both will be dictated by clinical experience of one skilled in the art, where different diseases are treated with different dosages and different agents. For exemplary purposes only, the following dosages of chemotherapeutic agents may be used to treat the following diseases. In treating glioblastoma, the cytotoxin temozolamide may be used. In treating melanoma, the cytotoxin melphalan or temozolamide may be used. In treating pancreatic cancer, the cytotoxin gemcitabine may be used. In treating breast cancer, the cytotoxin gemcitabine may be used. In treating colon cancer, the cytotoxin irinotecan or 5-fluorouracil may be used.
This interlaced therapy, i.e. administration of cell cycle inhibitors followed by administration of a dosage of at least one chemotherapeutic agent, a dosage of radiation, or a dosage of both can be used to reduce the progression, proliferation or growth of a disease or condition, as explained more thoroughly in Examples 4 and 5 below. In using this interlaced therapy, the same dosage of at least one chemotherapeutic agent, dosage of radiation, or dosage of both is more effective as compared to a chemotherapeutic or radiation dosage when used alone.
To measure the correspondence between calcium influx inhibition and progression or proliferation, the ability of several chemical agents to inhibit calcium influx was plotted against the ability of the same agent to inhibit proliferation, as can be seen in
Cell cycle analysis was performed using flow cytometry and BUdR staining. In
Pancreatic cancers resected from patients were immediately transplanted into the flanks of nude mice and maintained by serial, in vivo passage. Transplanted tumors were implanted at a volume of about 100 mm3 and allowed to grow to 200 to 300 mm3 before initiation of treatment. Mice bearing the PANC 219 tumor were either left untreated or treated with mibefradil at 65 mg/kg p.o. b.i.d. (n=10 in each group). Tumor growth was normalized to the size measured at the start of treatment. These results are shown in
Studies of interlaced therapy for human glioblastoma in a murine xenograft model using the D54 cell line were conducted. Mice bearing subcutaneous implants of D54 tumors, which were allowed to become established at a volume of about 100 mm3, were treated with mibefradil at 40 mg/kg p.o. q.i.d. for 7 days or left untreated. On day seven, all animals received the S phase cytotoxin temozolamide at a dose of 25% of the LD10 over five days. Following two days of no treatment, mibefradil was re-started at a dose of 35 mg/kg p.o. q.i.d. in the group of mice which were originally treated with mibefradil. On day 20, the mean tumor volume in the temozolamide only group of mice was 173 mm3 as compared to the temozolamide plus mibefradil group of mice, whose mean tumor volume was 102 mm3 (p=0.0485; n=10/group; Student's pooled, two tailed t-test). A pooled, two tailed. Student's t-test over all seven tumor volume measurements yielded p=0.0329. There were no animals that were euthanized in either group due to tumor size. The mean volume in the control group, which received no intervention, was 1214 mm3 with three animals euthanized because of tumor size.
Further studies of interlaced therapy for human glioblastoma in a murine xenograft model using the D54 cell line were conducted. Mice bearing subcutaneous implants of D54 tumors, which were allowed to become established, were treated with mibefradil at 40 mg/kg p.o. q.i.d. for 7 days or left untreated. On day seven, all animals received the S phase cytotoxin temozolamide at a dose of 25% of the LD10 over five days. Following two days of no treatment, mibefradil was re-started at a dose of 35 mg/kg p.o. q.i.d. in the group of mice which were originally treated with mibefradil. Following five days of mibefradil treatment, temozolamide was again administered for 5 days, but at a dose that is 10% of LD10, because the cytotoxin had made the tumors in six of twenty mice too small to measure following the first round of cytotoxin treatment. The results are shown below in
Filing Document | Filing Date | Country | Kind | 371c Date |
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PCT/US2010/037437 | 6/4/2010 | WO | 00 | 12/2/2011 |
Number | Date | Country | |
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61184658 | Jun 2009 | US |