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PROCESSING INVITRO OF AN ABASIC SITE REACTED WITH METHOXYAMINE - A NEW ASSAY FOR THE DETECTION OF ABASIC SITES FORMED INVIVO

被引:70
作者
ROSA, S
FORTINI, P
KARRAN, P
BIGNAMI, M
DOGLIOTTI, E
机构
[1] IST SUPER SANITA,COMPARAT TOXICOL & ECOTOXICOL LAB,VIALE REGINA ELENA 299,I-00161 ROME,ITALY
[2] IMPERIAL CANC RES FUND,CLARE HALL LABS,S MIMMS EN6 3LD,HERTS,ENGLAND
来源
NUCLEIC ACIDS RESEARCH | 1991年 / 19卷 / 20期
关键词
D O I
10.1093/nar/19.20.5569
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
In this study we demonstrate that the different substrate recognition properties of bacterial and human AP endonucleases might be used to quantify and localize apurinic (AP) sites formed in DNA in vivo. By using a model oligonucleotide containing a single AP site modified with methoxyamine (MX), we show that endonuclease III and IV of E. coli are able to cleave the alkoxyamine-adducted site whereas a partially purified HeLa AP endonuclease and crude cell-free extracts from HeLa cells are inhibited by this modification. In addition MX-modified AP sites in a DNA template retain their ability to block DNA synthesis in vitro. Since MX can efficiently react with AP sites formed in mammalian cells in vivo we propose that the MX modified abasic sites thus formed can be quantitated and localized at the level of the individual gene by subsequent site specific cleavage by either E. coli endonuclease III or IV in vitro.
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页码:5569 / 5574
页数:6
相关论文
共 37 条
[1]   BACTERIOPHAGE-T4 AND MICROCOCCUS-LUTEUS UV ENDONUCLEASES ARE NOT ENDONUCLEASES BUT BETA-ELIMINATION AND SOMETIMES BETA,DELTA-ELIMINATION CATALYSTS [J].
BAILLY, V ;
SENTE, B ;
VERLY, WG .
BIOCHEMICAL JOURNAL, 1989, 259 (03) :751-759
[2]   ESCHERICHIA-COLI ENDONUCLEASE-III IS NOT AN ENDONUCLEASE BUT A BETA-ELIMINATION CATALYST [J].
BAILLY, V ;
VERLY, WG .
BIOCHEMICAL JOURNAL, 1987, 242 (02) :565-572
[3]   O-6-METHYLGUANINE IN THE SV40 ORIGIN OF REPLICATION INHIBITS BINDING BUT INCREASES UNWINDING BY VIRAL LARGE T-ANTIGEN [J].
BIGNAMI, M ;
LANE, DP .
NUCLEIC ACIDS RESEARCH, 1990, 18 (13) :3785-3793
[4]   DNA-REPAIR IN AN ACTIVE GENE - REMOVAL OF PYRIMIDINE DIMERS FROM THE DHFR GENE OF CHO CELLS IS MUCH MORE EFFICIENT THAN IN THE GENOME OVERALL [J].
BOHR, VA ;
SMITH, CA ;
OKUMOTO, DS ;
HANAWALT, PC .
CELL, 1985, 40 (02) :359-369
[5]  
BOHR VA, 1987, CANCER RES, V47, P6426
[6]   CODING PROPERTIES OF POLY(DEOXYCYTIDYLIC ACID) TEMPLATES CONTAINING URACIL OR APYRIMIDINIC SITES - INVITRO MODULATION OF MUTAGENESIS BY DEOXYRIBONUCLEIC-ACID REPAIR ENZYMES [J].
BOITEUX, S ;
LAVAL, J .
BIOCHEMISTRY, 1982, 21 (26) :6746-6751
[7]   REACTION OF APURINIC ACID WITH ALDEHYDE REAGENTS [J].
COOMBS, MM ;
LIVINGSTON, DC .
BIOCHIMICA ET BIOPHYSICA ACTA, 1969, 174 (01) :161-+
[8]   THE ENZYMOLOGY OF APURINIC APYRIMIDINIC ENDONUCLEASES [J].
DOETSCH, PW ;
CUNNINGHAM, RP .
MUTATION RESEARCH, 1990, 236 (2-3) :173-201
[9]   EVIDENCE FOR AP SITE FORMATION RELATED TO DNA-OXYGEN ALKYLATION IN CHO CELLS TREATED WITH ETHYLATING AGENTS [J].
FORTINI, P ;
BIGNAMI, M ;
DOGLIOTTI, E .
MUTATION RESEARCH, 1990, 236 (01) :129-137
[10]   DNA DEOXYRIBOPHOSPHODIESTERASE [J].
FRANKLIN, WA ;
LINDAHL, T .
EMBO JOURNAL, 1988, 7 (11) :3617-3622
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