学术探索
学术期刊
新闻热点
数据分析
智能评审

HOW SENSITIVE IS PCR-SSCP

被引:426
作者
HAYASHI, K
YANDELL, DW
机构
[1] KYUSHU UNIV,INST GENET INFORMAT,DIV GENOME ANAL,FUKUOKA 812,JAPAN
[2] MASSACHUSETTS EYE & EAR INFIRM,DEPT OPHTHALMOL,BOSTON,MA 02114
来源
HUMAN MUTATION | 1993年 / 2卷 / 05期
关键词
MUTATIONAL ANALYSIS; POLYMERASE CHAIN REACTION (PCR); SINGLE-STRAND CONFORMATION POLYMORPHISM (SSCP); DNA TESTING;
D O I
10.1002/humu.1380020503
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
Single-strand conformation polymorphism analysis (SSCP) is a rapid method for detection of minor sequence changes in polymerase chain reaction-amplified DNA. Since the first reported use of SSCP in 1989 (Orita et al., 1989), this tehnique has been used widely to detect mutations in oncogenes, tumor suppressor genes, and genes responsible for genetic diseases. Published mutations that have been detected using this technique include base substitutions, small insertions and deletions, and rearrangements. This technique has also been applied for the detection of DNA polymorphisms at various loci of the human genome (reviewed by Hayashi, 1991; Hayashi, 1993). However, many factors can influence the sensitivity of SSCP, and its optimization is highly empirical. In this review, we estimate the percentage of mutations that can be detected by this technique under various controlled conditions, and describe some critical elements affecting sensitivity. (C) 1993 Wiley-Liss, Inc.
引用
收藏
页码:338 / 346
页数:9
相关论文
共 42 条
[31]   PRIMER-DIRECTED ENZYMATIC AMPLIFICATION OF DNA WITH A THERMOSTABLE DNA-POLYMERASE [J].
SAIKI, RK ;
GELFAND, DH ;
STOFFEL, S ;
SCHARF, SJ ;
HIGUCHI, R ;
HORN, GT ;
MULLIS, KB ;
ERLICH, HA .
SCIENCE, 1988, 239 (4839) :487-491
[32]   SCREENING FOR MUTATIONS BY RNA SINGLE-STRAND CONFORMATION POLYMORPHISM (RSSCP) - COMPARISON WITH DNA-SSCP [J].
SARKAR, G ;
YOON, HS ;
SOMMER, SS .
NUCLEIC ACIDS RESEARCH, 1992, 20 (04) :871-878
[33]   DIDEOXY FINGERPRINTING (DDF) - A RAPID AND EFFICIENT SCREEN FOR THE PRESENCE OF MUTATIONS [J].
SARKAR, G ;
YOON, HS ;
SOMMER, SS .
GENOMICS, 1992, 13 (02) :441-443
[34]   ATTACHMENT OF A 40-BASE-PAIR G+C-RICH SEQUENCE (GC-CLAMP) TO GENOMIC DNA FRAGMENTS BY THE POLYMERASE CHAIN-REACTION RESULTS IN IMPROVED DETECTION OF SINGLE-BASE CHANGES [J].
SHEFFIELD, VC ;
COX, DR ;
LERMAN, LS ;
MYERS, RM .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1989, 86 (01) :232-236
[35]  
SHEFFIELD VC, 1993, IN RPESS GENOMICS
[36]   ALLELE-SPECIFIC POLYMERASE CHAIN-REACTION - A METHOD FOR AMPLIFICATION AND SEQUENCE DETERMINATION OF A SINGLE COMPONENT AMONG A MIXTURE OF SEQUENCE VARIANTS [J].
SUZUKI, Y ;
SEKIYA, T ;
HAYASHI, K .
ANALYTICAL BIOCHEMISTRY, 1991, 192 (01) :82-84
[37]  
SUZUKI Y, 1990, ONCOGENE, V5, P1037
[38]  
TOGUCHIDA J, 1992, CANCER RES, V52, P1
[39]   THE USE OF SYNTHETIC OLIGONUCLEOTIDES AS HYBRIDIZATION PROBES .2. HYBRIDIZATION OF OLIGONUCLEOTIDES OF MIXED SEQUENCE TO RABBIT BETA-GLOBIN DNA [J].
WALLACE, RB ;
JOHNSON, MJ ;
HIROSE, T ;
MIYAKE, T ;
KAWASHIMA, EH ;
ITAKURA, K .
NUCLEIC ACIDS RESEARCH, 1981, 9 (04) :879-894
[40]   DETECTING SINGLE BASE SUBSTITUTIONS AS HETERODUPLEX POLYMORPHISMS [J].
WHITE, MB ;
CARVALHO, M ;
DERSE, D ;
OBRIEN, SJ ;
DEAN, M .
GENOMICS, 1992, 12 (02) :301-306
12345