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A comparison of Direct sequencing,Pyrosequencing,High resolution melting analysis,TheraScreen DxS,and the K-ras StripAssay for detecting KRAS mutations in non small cell lung carcinomas
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نویسنده
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jancik s. ,drabek j. ,berkovcova j. ,xu y.z. ,stankova m. ,klein j. ,kolek v. ,skarda j. ,tichy t. ,grygarkova i. ,radzioch d. ,hajduch m.
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منبع
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journal of experimental and clinical cancer research - 2012 - دوره : 31 - شماره : 1
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چکیده
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Background: it is mandatory to confirm the absence of mutations in the kras gene before treating metastatic colorectal cancers with epidermal growth factor receptor inhibitors,and similar regulations are being considered for non-small cell lung carcinomas (nsclc) and other tumor types. routine diagnosis of kras mutations in nsclc is challenging because of compromised quantity and quality of biological material. although there are several methods available for detecting mutations in kras,there is little comparative data regarding their analytical performance,economic merits,and workflow parameters. methods. we compared the specificity,sensitivity,cost,and working time of five methods using 131 frozen nsclc tissue samples. we extracted genomic dna from the samples and compared the performance of sanger cycle sequencing,pyrosequencing,high-resolution melting analysis (hrm),and the conformité européenne (ce)-marked therascreen dxs and k-ras stripassay kits. results and conclusions. our results demonstrate that therascreen dxs and the stripassay,in that order,were most effective at diagnosing mutations in kras. however,there were still unsatisfactory disagreements between them for 6.1% of all samples tested. despite this,our findings are likely to assist molecular biologists in making rational decisions when selecting a reliable,efficient,and cost-effective method for detecting kras mutations in heterogeneous clinical tumor samples. © 2012 jancik et al.; licensee biomed central ltd.
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کلیدواژه
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Genotyping; KRAS - Kiras2 kristen rat sarcoma viral oncogene homolog; NSCLC - Non-small cell lung cancer; SNP - single nucleotide polymorphism
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آدرس
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laboratory of experimental medicine,palacky university,university hospital in olomouc,olomouc, Czech Republic, laboratory of experimental medicine,palacky university,university hospital in olomouc,olomouc,czech republic,intellmed ltd,science and technology park of palacky university,olomouc, Czech Republic, laboratory of experimental medicine,palacky university,university hospital in olomouc,olomouc, Czech Republic, departments of experimental medicine and human genetics,mcgill university,montreal,qc, Canada, laboratory of experimental medicine,palacky university,university hospital in olomouc,olomouc,czech republic,institute of applied biotechnologies,prague, Czech Republic, 1st department of surgery,palacky university,university hospital in olomouc,olomouc, Czech Republic, department of pneumology and tuberculosis,palacky university,university hospital in olomouc,olomouc, Czech Republic, laboratory of molecular pathology,palacky university,university hospital in olomouc,olomouc, Czech Republic, laboratory of molecular pathology,palacky university,university hospital in olomouc,olomouc, Czech Republic, department of pneumology and tuberculosis,palacky university,university hospital in olomouc,olomouc, Czech Republic, departments of experimental medicine and human genetics,mcgill university,montreal,qc, Canada, laboratory of experimental medicine,palacky university,university hospital in olomouc,olomouc,czech republic,intellmed ltd,science and technology park of palacky university,olomouc, Czech Republic
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Authors
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