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Method of Treating Cancer by Inhibition of DNA Repair Proteins

a dna repair and cancer technology, applied in the field of cancer therapy, can solve the problems of inability to detect dna repair proteins,

Inactive Publication Date: 2017-01-19
SARISSA
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

Although necessary to confer a selective advantage to cancer cells, excessive instability in the cancer cell genome is suggested to be incompatible with cell viability.
Covalent binding of drugs to DNA or other interactions that interfere with transcription and / or replication initiates a series of events that, although intended to rescue the cell for further proliferation, may eventually lead to cell death.
However, PARP is also involved in repair pathways that are independent of BRCA1 and BRCA2 pathways and that tend to be more error-prone (8).
In this case, repair is very sensitive to inhibitors of PARP, and cells tend to accumulate replication-generated errors that would normally be repaired immediately, leading eventually to cell cycle arrest and cell death (8).
Full-length antisense mRNA expression vectors are currently not of potential clinical use.

Method used

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  • Method of Treating Cancer by Inhibition of DNA Repair Proteins
  • Method of Treating Cancer by Inhibition of DNA Repair Proteins
  • Method of Treating Cancer by Inhibition of DNA Repair Proteins

Examples

Experimental program
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Effect test

example 1

Design of Antisense Oligonucleotides to BRCA2

[0204]Three antisense oligonucleotides (OLIGOs) to BRCA2 were designed. The first OLIGO, named BR1, was based on the sequence of a siRNA (siRNA J-003462-08-0005) commercially available from Dharmacon Inc. (Lafayette, Colo.). BR1 has the following sequence:

[SEQ ID NO: 17]5′-guaucuCTTGACGTuccuua-3′

(40% GC content)

[0205]Wherein the lower case letters represent 2′O-methyl RNA and the upper case letters represent DNA. The OLIGO was fully phosphorothioated. The BR1 OLIGO targets the coding region, bases 7241-7259 of the BRCA2 mRNA, specifically, the following BRCA2 mRNA sequence:

[SEQ ID NO: 18]5′-UAAGGAACGUCAAGAGAUAC-3′

[0206]Two other OLIGOs, BR2 and BR3, were designed using the NCI web-based BLAST program. The program was asked to design sequence-specific PCR primers. Pairs of primers were obtained for the coding region and the 3′-UTR of the BRCA mRNA. Based on these sequences, antisense sequences were designed and their specificity to BRCA2 m...

example 2

Inhibition of Proliferation of A549B Cells by an Antisense Oligonucleotide to BRCA2

[0213]The effect of an antisense oligonucleotide against BRCA2 on proliferation of non-small cell lung cancer (NSCLC) cells was tested. The BRCA2 antisense oligonucleotide tested in this experiment was BR1, described below. The experiment was carried out as follows.

Cell Culture Techniques.

[0214]Cell culture medium was purchased from Wisent, Inc. (St-Bruno, Quebec, Canada). Fetal bovine serum and Lipofectamine 2000 were purchased from Invitrogen, Inc. Cell culture plasticware was obtained from Invitrogen (Life technologies, Burlington, Ontario, Canada), Fisher Scientific (Unionville, Ontario), and VWR Canlab (Mississauga, Ontario).

[0215]Cultured cell lines were maintained in minimum essential medium a with nucleosides plus 10% fetal bovine serum and penicillin (50 units / mL) / streptomycin (50 mg / L) (growth medium). Cultures were incubated in a humidified atmosphere of 5% CO2 at 37° C. Cultured cell lines...

example 3

Inhibition of Proliferation of A549B Cells Pretreated With an Antisense Oligonucleotide to BRCA2 by Olaparib

[0221]This experiment examined the effect of pre-treating A549b cells with the BRCA2 antisense oligonucleotide BR1 on the ability of the PARP (poly(ADP ribose) polymerase) inhibitor olaparib to inhibit proliferation of these cells. These experiments were carried out as follows.

[0222]Cells were cultured and maintained as described in Example 2. The antisense oligonucleotide sequences used were also as described in Example 2.

[0223]Cells were treated with OLIGOs and / or olaparib as follows.

[0224]OLIGOs were introduced into cells with the use of Lipofectamine 2000 (LFA2K) (Invitrogen, Burlington, Ontario, Canada). OLIGOs were mixed with LFA2K at a ratio of 0.2 μg / ml per 10 nM OLIGO. The mixture was prepared at 11× the final concentration to which cells were exposed, so that 200 μL was added to 2 mL of medium in which cells were plated. After incubating at room temperature for 20 mi...

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Abstract

Methods of treating cancer using antisense oligonucleotides directed against DNA double-strand break repair proteins such as BRCA2 or RAD51 are provided. The antisense oligonucleotides can he used alone, in tandem or in combination with other cancer therapies, in particular with therapies that lead to DNA damage, inhibition of DNA repair or inhibition of DNA synthesis, such as radiation, platinum drugs, alkylating agents, PARP inhibitors, or inhibitors of thymidylate synthase.

Description

FIELD OF THE INVENTION[0001]The present invention relates to the field of cancer therapy and, in particular, to the use of antisense oligonucleotides directed against DNA repair proteins involved in the repair of double strand DNA breaks in the treatment of cancer.BACKGROUND OF THE INVENTION[0002]Cancer is characterized by genetic instability both at the chromosomal level and at the nucleotide level. The acquisition of certain mutations confers a selective advantage to the cancer cells and is critical in cancer progression. A diverse array of defects in both DNA polymerases and DNA repair enzymes appears to contribute to the increased genetic instability observed in cancer cells (Hanahan et al, 2011, Cell, 144: 646-674). Although necessary to confer a selective advantage to cancer cells, excessive instability in the cancer cell genome is suggested to be incompatible with cell viability. Treatment of cancer by increasing the genetic instability of cancer cells beyond the threshold ov...

Claims

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Application Information

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Patent Type & Authority Applications(United States)
IPC IPC(8): C12N15/113A61K31/502A61K31/513A61K31/198A61K31/282A61K31/713A61K33/24A61K33/243
CPCC12N15/1135C12N2310/14A61K31/502A61K33/24C12N15/1137A61K31/198A61K31/282C12N15/113A61K31/513C12N2310/11C12N2310/341C12N2320/31C12N2310/315C12N2310/321A61K31/713A61K31/7088A61K31/7105A61K31/7115C12N2310/322C12N2310/346C12Y201/01045A61P35/00A61K33/243C12N2310/3521C12N2310/3525A61K2300/00
Inventor VINCENT, MARKFERGUSON, PETER J.RYTELEWSKI, MATEUSZ
Owner SARISSA
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