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人类基因组中间质端粒序列的不稳定性。

Instability of interstitial telomeric sequences in the human genome.

作者信息

Mondello C, Pirzio L, Azzalin C M, Giulotto E

机构信息

Istituto di Genetica Biochimica ed Evoluzionistica, CNR, Via Abbiategrasso 207, Pavia, 27100, Italy.

出版信息

Genomics. 2000 Sep 1;68(2):111-7. doi: 10.1006/geno.2000.6280.

DOI:10.1006/geno.2000.6280
PMID:10964508
Abstract

The length variability of four human interstitial telomeric sequences (ITs) is described. Three of the ITs contain short telomeric stretches ranging between 53 and 84 bp and are localized in 21q22, 2q31, and 7q36; the fourth IT derives from the subtelomeric domain of chromosome 6p and contains a tract of a few hundred basepairs of exact and degenerate repeats. Using primers flanking the repeats, we amplified the genomic DNA from unrelated individuals and from family members, and we found that all the loci are polymorphic. At the 21q22 IT locus, two equally frequent alleles were found, while the number of alleles at the 2q31, 7q36, and 6pter IT loci was 8, 6, and 4, respectively. Sequence analysis revealed that in the three loci containing short ITs the alleles differ from one another for multiples of the hexanucleotide; it is likely that the mechanism leading to the polymorphism is DNA polymerase slippage. These loci were also unstable in gastric tumor cells characterized by microsatellite instability. At the 6pter IT locus, the four alleles range in length from about 500 to about 700 bp; this variability is probably due to unequal exchange or gene conversion. Our data indicate that stretches of exact internal telomeric repeats can be highly unstable, like microsatellites with shorter units, and that they can be useful polymorphic markers for linkage analysis, for forensic applications, and for the detection of genetic instability in tumors.

摘要

本文描述了四个人类间质端粒序列(ITs)的长度变异性。其中三个ITs包含长度在53至84 bp之间的短端粒片段,分别定位于21q22、2q31和7q36;第四个ITs来源于6p染色体的亚端粒区域,包含几百个碱基对的精确和简并重复序列。我们使用重复序列两侧的引物,从无关个体和家庭成员中扩增基因组DNA,发现所有位点均具有多态性。在21q22 IT位点,发现了两个频率相同的等位基因,而在2q31、7q36和6pter IT位点的等位基因数量分别为8个、6个和4个。序列分析表明,在三个包含短ITs的位点,等位基因之间相差六核苷酸的倍数;导致多态性的机制可能是DNA聚合酶滑动。这些位点在具有微卫星不稳定性的胃肿瘤细胞中也不稳定。在6pter IT位点,四个等位基因的长度范围约为500至700 bp;这种变异性可能是由于不等交换或基因转换。我们的数据表明,精确的内部端粒重复序列片段可能像较短单元的微卫星一样高度不稳定,并且它们可作为有用的多态性标记用于连锁分析、法医应用以及检测肿瘤中的遗传不稳定性。

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