EVALUATION OF GENE DELETIONS BY QUANTITATIVE POLYMERASE CHAIN-REACTION - EXPERIENCE WITH THE ALPHA-THALASSEMIA MODEL

被引:0
作者
BORRIELLO, F
WEINBERG, DS
MUTTER, GL
机构
[1] BRIGHAM & WOMENS HOSP, DEPT PATHOL, BOSTON, MA 02115 USA
[2] HARVARD UNIV, SCH MED, BOSTON, MA USA
来源
DIAGNOSTIC MOLECULAR PATHOLOGY | 1994年 / 3卷 / 04期
关键词
POLYMERASE CHAIN REACTION; THALASSEMIA; MOLECULAR DIAGNOSTICS; QUANTITATION; ALPHA-GLOBIN;
D O I
暂无
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 order to evaluate the feasibility of using quantitative polymerase chain reaction (PCR) to evaluate gene dosage, we developed an assay to detect alpha-globin genes, which are frequently deleted in alpha-thalassemia patients. In this quantitative assay alpha-1 and alpha-2 globin consensus regions are coamplified by one oligonucleotide pair, along with a second primer pair targeting a single-copy reference gene, namely, tumor necrosis factor alpha, or TNF-alpha. A series of DNA samples titrating alpha-globin against TNF-alpha DNA have a strong linear relationship between template ratios and product ratios (r > 0.98). Minimal sequence divergence (91% homology) between alpha-1 and alpha-2, internal to the identical primer annealing sites, results in a lower amplification efficiency for alpha-1, to 94% of alpha-2 for each cycle. Furthermore, when applied to a variety of individual DNA samples, the signal ratios of alpha-globin to TNF-alpha were far more variable than previously observed for titrated control DNA. We conclude that DNA isolates from different individuals may have idiosyncratic changes in amplification efficiency owing to polymorphic sequence variation and/or variable presence of unidentified contaminants. Despite these potentially confounding factors, however, we were able to identify by quantitative PCR a single gene deletion later confirmed by Southern blot analysis in 20 individual DNA samples.
引用
收藏
页码:246 / 254
页数:9
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