Wednesday, August 22, 2012

PCR-based screening for the EML4-ALK oncogene in lung cancer?

http://www.ncbi.nlm.nih.gov/pubmed/22908099


 2012 Aug 20. [Epub ahead of print]

A prospective PCR-based screening for the EML4-ALK oncogene in non-small cell lung cancer.

Source

Division of Functional Genomics, Jichi Medical University.

Abstract

PURPOSE:

EML4-ALK is a lung cancer oncogene, and ALK inhibitors show marked therapeutic efficacy for tumors harboring this fusion gene. It remains unsettled, however, how the fusion gene should be detected in specimens other than formalin-fixed, paraffin-embedded tissue. We here tested whether reverse transcription (RT) and PCR-based detection of EML4-ALK is a sensitive and reliable approach.

EXPERIMENTAL DESIGN:

We developed a multiplex RT-PCR system to capture ALK fusion transcripts and applied this technique to our prospective, nationwide cohort of non-small cell lung cancer in Japan.

RESULTS:

During February to December 2009, we collected 916 specimens from 853 patients, quality filtering of which yielded 808 specimens of primary non-small cell lung cancer from 754 individuals. Screening for EML4-ALK and KIF5B-ALK with our RT-PCR system identified EML4-ALK transcripts in 36 samples (4.46%) from 32 individuals (4.24%). The RT-PCR products were detected in specimens including bronchial washing fluid (n = 11), tumor biopsy (n = 8), resected tumor (n = 7), pleural effusion (n = 5), sputum (n = 4), and metastatic lymph node (n = 1). The results of RT-PCR were concordant with those of sensitive immunohistochemistry with ALK antibodies.

CONCLUSIONS:

Multiplex RT-PCR was confirmed to be a reliable technique for detection of ALK fusion transcripts. We propose that diagnostic tools for EML4-ALK should be selected in a manner dependent on the available specimen types. FISH and sensitive immunohistochemistry should be applied to formalin-fixed, paraffin-embedded tissue, but multiplex RT-PCR is appropriate for other specimen types.

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