Title of article :
Establishment and molecular cytogenetic characterization of non–small cell lung cancer cell line KU-T1 by multicolor fluorescence in situ hybridization, comparative genomic hybridization, and chromosome microdissection
Author/Authors :
Kume، نويسنده , , Motohiko and Taguchi، نويسنده , , Takahiro and Okada، نويسنده , , Hironobu and Anayama، نويسنده , , Takashi and Tominaga، نويسنده , , Akira and Shuin، نويسنده , , Taro and Sasaguri، نويسنده , , Shiro، نويسنده ,
Issue Information :
روزنامه با شماره پیاپی سال 2007
Pages :
9
From page :
93
To page :
101
Abstract :
A human lung adenocarcinoma cell line, designated KU-T1, was established from a Japanese man in Kochi Medical School. Conventional banding and multicolor fluorescence in situ hybridization (M-FISH) analyses of KU-T1 cells revealed a hyperdiploid chromosomal constitution and complex karyotypes. Comparative genomic hybridization showed several chromosomal copy number changes, and five regions that were highly amplified. Two of the five highly amplified regions, 1q and 3q, were identified from distributions of DNA sequences on a metaphase cell by FISH using chromosome microdissection-generated probes hybridized to 1q32∼q34 and 3q26∼q28, respectively. The 3q probe depicted a homogeneously staining region (hsr) in a derivative chromosome 3 of KU-T1. An hsr probe was regenerated by chromosome microdissection and was hybridized back to KU-T1 and normal metaphases. This hybridization experiment confirmed the probe derived from an hsr and indicated original locations of DNA sequences of hsr on normal chromosome 3. Intense hybridized signals shown at three loci (3p12, 3q26.3, and 3q28) suggests that oncogenes may be involved in the hsr formation. The present study provides a comprehensive analysis of the chromosomal abnormalities, including hsr formation and related oncogenes, in the KU-T1 cell line.
Journal title :
Cancer Genetics and Cytogenetics
Serial Year :
2007
Journal title :
Cancer Genetics and Cytogenetics
Record number :
1828787
Link To Document :
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