EFFICIENT CDNA CLONING BY DIRECT PHENOTYPIC CORRECTION OF A MUTANT HUMAN CELL-LINE (HPRT-) USING AN EPSTEIN-BARR VIRUS-DERIVED CDNA EXPRESSION VECTOR

被引：9

作者：

BELT, PBGM

JONGMANS, W

DEWIT, J

HOEIJMAKERS, JHJ

VANDEPUTTE, P

BACKENDORF, C

机构：

[1] LEIDEN UNIV,GORLAEUS LABS,DEPT BIOCHEM,MOLEC GENET LAB,POB 9502,2300 AL LEIDEN,NETHERLANDS

[2] ERASMUS UNIV,DEPT CELL BIOL & GENET,3000 DR ROTTERDAM,NETHERLANDS

来源：

NUCLEIC ACIDS RESEARCH | 1991年 / 19卷 / 18期

关键词：

D O I：

10.1093/nar/19.18.4861

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

Human cells are, in general, poor recipients of foreign DNA, which has severely hampered the cloning of genes by direct phenotypic correction of deficient human cell lines after DNA mediated gene transfer. In this communication a methodology is presented which largely circumvents this problems. The method relies on the use of a recently developed episomal Epstein - Barr-virus-derived cDNA expression vector (Belt et al. (1989) Gene 84, 407 - 417). The cloning of hypoxanthine phosphoribosyltransferase (HPRT) cDNA, corresponding to a low abundant mRNA in wild type cells is used as a model system. Size fractionated poly (A)+ RNA from wild type cells, which resulted in an approximately 10 fold enrichment in HPRT mRNA, was used to construct a cDNA library of 25,000 independent clones in the pECV25 vector. An HPRT deficient human cell line was transfected and subsequently selected with hygromycin B for DNA uptake. In a small scale experiment only 7000 hygromycin B(R) transfectants were sufficient to isolate 2 independent HAT(R) clones which were shown to replicate episomes harbouring HPRT cDNA. The first insert had a 5' untranslated region (UTR) and a 3' UTR perfectly in agreement with published data. The second cDNA clone harboured an unusually long 5' UTR and a shorter 3' UTR due to alternative polyadenylation of the HPRT transcript which has not been previously recognized.

引用

页码：4861 / 4866

页数：6

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