CFTR ILLEGITIMATE TRANSCRIPTION IN LYMPHOID-CELLS - QUANTIFICATION AND APPLICATIONS TO THE INVESTIGATION OF PATHOLOGICAL TRANSCRIPTS

被引:32
作者
FONKNECHTEN, N [1 ]
CHELLY, J [1 ]
LEPERCQ, J [1 ]
KAHN, A [1 ]
KAPLAN, JC [1 ]
KITZIS, A [1 ]
CHOMEL, JC [1 ]
机构
[1] INST COCHIN GENET MOLEC,BIOCHIM GENET LAB,F-75014 PARIS,FRANCE
关键词
D O I
10.1007/BF00219336
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
Since the isolation of the cystic fibrosis transmembrane conductance regulator gene (CFTR) and the characterization of the main mutation (DELTA-F508) in 1989, a large number of rare mutations has been found. Full screening of the CFTR gene is difficult because it is split into 27 exons covering 250 kb of genomic DNA. This gene is essentially expressed in the lung and intestinal tract, neither of which are easily accessible for routine investigations. The recent description of a faint transcription of highly tissue-specific genes in any cell, a phenomenon known as illegitimate transcription, would facilitate the research of mutations and the characterization of truncated m-RNA caused by splicing mutations. Using the polymerase chain reaction on cDNA (cDNA-PCR), we detected transcripts of the CFTR gene in lymphocytes and lymphoblast cells at a very low level (about 300 times less than in lung or intestine). This strategy allowed us to obtain a sufficient amount of cDNA-PCR product compatible with further molecular analyses. We have, therefore, analyzed a cDNA fragment overlapping exons 10 and 11 by polyacrylamide gel electrophoresis and direct sequencing, and detected the DELTA-F508 mutation at this level. Our protocol can be generalized to the investigation of the total 4.5-kb CFTR coding sequence.
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页码:508 / 512
页数:5
相关论文
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