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小鼠t单倍型内的重组已经取代了t特异性DNA的重要片段。

Recombination within mouse t haplotypes has replaced significant segments of t-specific DNA.

作者信息

Wallace Lyle T, Erhart Mark A

机构信息

Department of Biological Sciences, Chicago State University, Chicago, IL 60628, USA.

出版信息

Mamm Genome. 2008 Apr;19(4):263-71. doi: 10.1007/s00335-008-9103-3. Epub 2008 Apr 1.

Abstract

Previous studies on the fourth inversion of the t complex, In17(4), suggest that loci near the center of this inversion have been subjected to segmental recombination during the past 1-2 million years. We have used a combination of PCR-based restriction site (PBR) analysis and DNA sequencing to perform a high-resolution analysis of a 2-million base pair (Mbp) segment in the middle of In17(4). We examined 21 restriction sites that are polymorphic between t haplotypes and their wild-type homologs, over nine distinct loci. In addition, we examined several other polymorphic sites through DNA sequence analysis of two of these nine loci. We analyzed several haplotypes in this way, including the "complete" t haplotypes tw2, t0, tw32, tw71, and tw75. We show that only tw32 is a true "complete" t haplotype; the remaining four t haplotypes have segments of wild-type DNA ranging from less than 100 bp to 2 Mbp. The sizes of these wild-type DNA segments are consistent with their being generated by gene-conversion events. The 2-Mbp segment is located in a region that may contain the t-complex distorter gene Tcd2. One of the nine loci examined in this study is Fgd2, a gene that has been proposed to encode Tcd2. Sequencing and PBR data show that at least a portion of the Fgd2 gene has been converted to the wild-type within tw71 and tw75mice.

摘要

以往对t复合体第四倒位In17(4)的研究表明,在过去的100万到200万年里,这个倒位中心附近的基因座经历了片段重组。我们结合基于聚合酶链反应的限制性位点(PBR)分析和DNA测序,对In17(4)中间一段200万个碱基对(Mbp)的片段进行了高分辨率分析。我们检测了21个在t单倍型及其野生型同源物之间具有多态性的限制性位点,分布在9个不同的基因座上。此外,我们通过对这9个基因座中的两个进行DNA序列分析,检测了其他几个多态性位点。我们以这种方式分析了几种单倍型,包括“完整”的t单倍型tw2、t0、tw32、tw71和tw75。我们发现只有tw32是真正的“完整”t单倍型;其余四种t单倍型含有长度从不到100 bp到2 Mbp不等的野生型DNA片段。这些野生型DNA片段的大小与由基因转换事件产生的大小一致。这个2 Mbp的片段位于一个可能包含t复合体畸变基因Tcd2的区域。本研究检测的9个基因座之一是Fgd2,有人提出该基因编码Tcd2。测序和PBR数据表明,在tw71和tw75小鼠中,至少部分Fgd2基因已转换为野生型。

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