Development and validation of the JAX Cancer Treatment Profile™ for detection of clinically actionable mutations in solid tumors

Ananda, Guruprasad; Mockus, Susan M.; Lundquist, Micaela; Spotlow, Vanessa; Simons, Allen K.; Mitchell, Talia; Stafford, Grace A.; Philip, Vivek M.; Stearns, Timothy M.; Srivastava, Anuj; Barter, Mary; Rowe, Lucy B.; Malcolm, Joan; Bult, Carol J.; Karuturi, R. Krishna Murthy; Karen, Rasmussen; Hinerfeld, Douglas

doi:10.1016/j.yexmp.2014.12.009

Cited by 31 publications

(31 citation statements)

References 25 publications

(25 reference statements)

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“…Among the 342 significantly altered genes, we also found previously known critical genetic drivers including TP53, ARID1A, PIK3CA, KRAS, MYC, FAT4, CTNNB1, and ERBB2 (SI Appendix, Table S9) (6,19). Using the JAX Cancer Treatment Profile analysis pipeline, we also identified clinically actionable mutations in 144 genes as candidate targets for clinical application (JAX-CTP; Dataset S3) (20).…”

Section: Significancementioning

confidence: 99%

Genomic alterations in BCL2L1 and DLC1 contribute to drug sensitivity in gastric cancer

Park

Cho

Kim

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

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Gastric cancer (GC) is the third leading cause of cancer-related deaths worldwide. Recent high-throughput analyses of genomic alterations revealed several driver genes and altered pathways in GC. However, therapeutic applications from genomic data are limited, largely as a result of the lack of druggable molecular targets and preclinical models for drug selection. To identify new therapeutic targets for GC, we performed array comparative genomic hybridization (aCGH) of DNA from 103 patients with GC for copy number alteration (CNA) analysis, and whole-exome sequencing from 55 GCs from the same patients for mutation profiling. Pathway analysis showed recurrent alterations in the Wnt signaling [APC, CTNNB1, and DLC1 (deleted in liver cancer 1)], ErbB signaling (ERBB2, PIK3CA, and KRAS), and p53 signaling/apoptosis [TP53 and BCL2L1 (BCL2-like 1)] pathways. In 18.4% of GC cases (19/103), amplification of the antiapoptotic gene BCL2L1 was observed, and subsequently a BCL2L1 inhibitor was shown to markedly decrease cell viability in BCL2L1-amplified cell lines and in similarly altered patient-derived GC xenografts, especially when combined with other chemotherapeutic agents. In 10.9% of cases (6/55), mutations in DLC1 were found and were also shown to confer a growth advantage for these cells via activation of Rho-ROCK signaling, rendering these cells more susceptible to a ROCK inhibitor. Taken together, our study implicates BCL2L1 and DLC1 as potential druggable targets for specific subsets of GC cases.gastric cancer | copy number alteration | whole-exome sequencing | patient-derived xenograft | druggable target G astric cancer (GC) is a highly prevalent malignancy and is the third leading cause of cancer-related deaths in the world (1). In unresectable and metastatic cases, the clinical outcome for this disease remains poor (median survival is 10-14 mo) (2), and other treatment options are often limited because of the lack of effective therapeutic approaches and molecular prognostic markers (2, 3). To date, with the exception of the application of trastuzumab [ERBB2 (ErbB2 receptor tyrosine kinase 2) antagonist] or ramucirumab [VEGFR2 (Vascular endothelial growth factor receptor 2) antagonist] for advanced GC cases (4, 5), drugs that target GC on a molecular level are limited.Recent genomic studies have demonstrated the heterogeneous genomic characteristics of GC (6-10). In addition, previous studies of patients with GC by whole-genome and whole-exome sequencing (WES) have identified frequent somatic mutations in tumor suppressors such as TP53, ARID1A, APC, and FAT4, and oncogenes including PI3KCA, KRAS, and RHOA (6-10). However, these findings, although academically meaningful, are far from ready for clinical applications, largely because of the lack of identified druggable molecular targets and the availability of reliable preclinical models for validation of potential target inhibitors.To identify novel therapeutic targets for GC, we explored genomic alterations in GC through an integrated genomic data set from WE...

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Section: Significancementioning

confidence: 99%

Genomic alterations in BCL2L1 and DLC1 contribute to drug sensitivity in gastric cancer

Park

Cho

Kim

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

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“…We identified somatic mutations by comparing mutations detected in tumor and blood samples and custom filters to extract the most likely candidates. Subsets of SNVs found in cancer-related genes (2,7,12,16,18,20,23,24,37,38,42) were randomly selected, and a two-step validation was performed to obtain a set of high-confidence somatic mutations. Optimization of parameters and filtering rules were performed according to the results of the validation.…”

Section: Data Analysis Workflowmentioning

confidence: 99%

<b>Optimizing an ion semiconductor sequencing data analysis method to identify somatic mutations in the genomes of cancer cells in clinical tissue </b><b>samples </b>

et al. 2016

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Identification of causal genomic alterations is an indispensable step in the implementation of personalized cancer medicine. Analytical methods play a central role in identifying such changes because of the vast amount of data produced by next generation sequencer. Most analytical techniques are designed for the Illumina platform and are therefore suboptimal for analyzing datasets generated by whole exome sequencing (WES) using the Ion Proton System. Accurate identification of somatic mutations requires the characterization of platform-dependent error profiles and genomic properties that affect the accuracy of sequence data as well as platform-oriented optimization of the pipeline. Therefore, we used the Ion Proton System to perform WES of DNAs isolated from tumor and matched control tissues of 1,058 patients with cancer who were treated at the Shizuoka Cancer Center Hospital. Among the initially identified candidate somatic single-nucleotide variants (SNVs), 10,279 were validated by manual inspection of the WES data followed by Sanger sequencing. These validated SNVs were used as an objective standard to determine an optimum cutoff value to improve the pipeline. Using this optimized pipeline analysis, 189,381 SNVs were identified in 1,101 samples. The analytical technique presented here is a useful resource for conducting clinical WES, particularly using semiconductor-based sequencing technology.

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“…In cases where multiple nucleotides are incorporated in a row, the intensity of the light fluoresces will dictate how many bases were added. 454's technology allowed for sequencing of longer reads, reaching up to 1 Kb, compared to some of the other available platforms at that time [24,25].…”

Section: Next Generation Sequencingmentioning

confidence: 99%

“…Taking Illumina's idea one step further, other companies have designed their own custom targeted panels which can then be developed as clinical tests to be offered to physicians. As an example, the Jackson Laboratory for Genomic Medicine offers a custom targeted sequencing panel, the JAX Cancer Treatment Profile TM (JAX-CTP TM ), which analyses 358 cancer-associated genes in a diverse subset of cancer types [24]. Accompanying the 358 gene panel, a targeted fusion detection assay is incorporated to detect gene fusions in 53 genes linked to solid tumors.…”

Section: Citationmentioning

confidence: 99%

A Comprehensive Evaluation of Solid Tumor Analysis in the Clinical Space

Kelly¹,

Ras²,

Helm³

2016

Next Generat Sequenc & Applic

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Solid tumors remain a major health concern with approximately 14 million new cases and 8.2 million cancerrelated deaths per year. Currently multimodality treatment regimens are being explored to make advances against this deadly disease. Tumors are characterized by genomic instability and tailored therapies are being considered based on genetic profiling of cancers, driving precision medicine. This review outlines the various genetic changes present in solid tumors, evaluates the technologies currently used for identification of variants and compares the large panels available for clinical utility and comprehensiveness.

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Development and validation of the JAX Cancer Treatment Profile™ for detection of clinically actionable mutations in solid tumors

Cited by 31 publications

References 25 publications

Genomic alterations in BCL2L1 and DLC1 contribute to drug sensitivity in gastric cancer

Genomic alterations in BCL2L1 and DLC1 contribute to drug sensitivity in gastric cancer

<b>Optimizing an ion semiconductor sequencing data analysis method to identify somatic mutations in the genomes of cancer cells in clinical tissue </b><b>samples </b>

A Comprehensive Evaluation of Solid Tumor Analysis in the Clinical Space

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