CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations

Molecular diagnostics has changed the way lung cancer patients are treated worldwide. Of several different testing methods available, PCR followed by directed sequencing and amplification refractory mutation system (ARMS) are the two most commonly used diagnostic methods worldwide to detect mutation...

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Autores principales: Ramteke, Manoj P., Patel, Kuldeep J, Godbole, Mukul, Vyas, Maulik, Karve, Kunal, Choughule, Anuradha, Prabhash, Kumar, Dutt, Amit
Formato: Online Artículo Texto
Lenguaje:English
Publicado: F1000Research 2016
Materias:
Method Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4830212/
https://www.ncbi.nlm.nih.gov/pubmed/27127615
http://dx.doi.org/10.12688/f1000research.6663.2
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author Ramteke, Manoj P.
Patel, Kuldeep J
Godbole, Mukul
Vyas, Maulik
Karve, Kunal
Choughule, Anuradha
Prabhash, Kumar
Dutt, Amit
author_facet Ramteke, Manoj P.
Patel, Kuldeep J
Godbole, Mukul
Vyas, Maulik
Karve, Kunal
Choughule, Anuradha
Prabhash, Kumar
Dutt, Amit
author_sort Ramteke, Manoj P.
collection PubMed
description Molecular diagnostics has changed the way lung cancer patients are treated worldwide. Of several different testing methods available, PCR followed by directed sequencing and amplification refractory mutation system (ARMS) are the two most commonly used diagnostic methods worldwide to detect mutations at  KRAS exon 2 and  EGFR kinase domain exons 18-21 in lung cancer. Compared to ARMS, the PCR followed by directed sequencing approach is relatively inexpensive but more cumbersome to perform. Moreover, with a limiting amount of genomic DNA from clinical formalin-fixed, paraffin-embedded (FFPE) specimens or fine biopsies of lung tumors, multiple rounds of PCR and sequencing reactions often get challenging. Here, we report a cost-effective single multiplex-PCR based method, CRE (for  Co-amplification of five  K RAS and  E GFR exons), followed by concatenation of the PCR product as a single linear fragment for direct sequencing. CRE is a robust protocol that can be adapted for routine use in clinical diagnostics with reduced variability, cost and turnaround time requiring a minimal amount of template DNA extracted from FFPE or fresh frozen tumor samples. As a proof of principle, CRE is able to detect the activating  EGFR L858R and T790M  EGFR mutations in lung cancer cell line and primary tumors.
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spelling pubmed-48302122016-04-27 CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations Ramteke, Manoj P. Patel, Kuldeep J Godbole, Mukul Vyas, Maulik Karve, Kunal Choughule, Anuradha Prabhash, Kumar Dutt, Amit F1000Res Method Article Molecular diagnostics has changed the way lung cancer patients are treated worldwide. Of several different testing methods available, PCR followed by directed sequencing and amplification refractory mutation system (ARMS) are the two most commonly used diagnostic methods worldwide to detect mutations at  KRAS exon 2 and  EGFR kinase domain exons 18-21 in lung cancer. Compared to ARMS, the PCR followed by directed sequencing approach is relatively inexpensive but more cumbersome to perform. Moreover, with a limiting amount of genomic DNA from clinical formalin-fixed, paraffin-embedded (FFPE) specimens or fine biopsies of lung tumors, multiple rounds of PCR and sequencing reactions often get challenging. Here, we report a cost-effective single multiplex-PCR based method, CRE (for  Co-amplification of five  K RAS and  E GFR exons), followed by concatenation of the PCR product as a single linear fragment for direct sequencing. CRE is a robust protocol that can be adapted for routine use in clinical diagnostics with reduced variability, cost and turnaround time requiring a minimal amount of template DNA extracted from FFPE or fresh frozen tumor samples. As a proof of principle, CRE is able to detect the activating  EGFR L858R and T790M  EGFR mutations in lung cancer cell line and primary tumors. F1000Research 2016-03-08 /pmc/articles/PMC4830212/ /pubmed/27127615 http://dx.doi.org/10.12688/f1000research.6663.2 Text en Copyright: © 2016 Ramteke MP et al. http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution Licence, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. The author(s) is/are employees of the US Government and therefore domestic copyright protection in USA does not apply to this work. The work may be protected under the copyright laws of other jurisdictions when used in those jurisdictions.
spellingShingle Method Article
Ramteke, Manoj P.
Patel, Kuldeep J
Godbole, Mukul
Vyas, Maulik
Karve, Kunal
Choughule, Anuradha
Prabhash, Kumar
Dutt, Amit
CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title_full CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title_fullStr CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title_full_unstemmed CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title_short CRE: a cost effective and rapid approach for PCR-mediated concatenation of KRAS and EGFR exons: Rapid way to detect EGFR and KRAS mutations
title_sort cre: a cost effective and rapid approach for pcr-mediated concatenation of kras and egfr exons: rapid way to detect egfr and kras mutations
topic Method Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4830212/
https://www.ncbi.nlm.nih.gov/pubmed/27127615
http://dx.doi.org/10.12688/f1000research.6663.2
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