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评估两种方法对雀形目动物 CE-SSCP 和 454 焦磷酸测序的主要组织相容性复合物 I 类基因分型。

Evaluation of two approaches to genotyping major histocompatibility complex class I in a passerine-CE-SSCP and 454 pyrosequencing.

机构信息

Institute of Vertebrate Biology, Academy of Sciences of the Czech Republic, Květná 8, 60365 Brno, Czech Republic.

出版信息

Mol Ecol Resour. 2012 Mar;12(2):285-92. doi: 10.1111/j.1755-0998.2011.03082.x. Epub 2011 Oct 24.

Abstract

Genes of the highly dynamic major histocompatibility complex (MHC) are directly linked to individual fitness and are of high interest in evolutionary ecology and conservation genetics. Gene duplication and positive selection usually lead to high levels of polymorphism in the MHC region, making genotyping of MHC a challenging task. Here, we compare the performance of two methods for MHC class I genotyping in a passerine with highly duplicated MHC class I genes: capillary electrophoresis-single-strand conformation polymorphism (CE-SSCP) analysis and 454 GS FLX Titanium pyrosequencing. According to our findings, the number of MHC variants (called alleles for simplicity) detected by CE-SSCP is significantly lower than detected by 454. To resolve discrepancies between the two methods, we cloned and Sanger sequenced a MHC class I amplicon for an individual with high number of alleles. We found a perfect congruence between cloning/Sanger sequencing results and 454. Thus, in case of multi-locus amplification, CE-SSCP considerably underestimates individual MHC diversity. However, numbers of alleles detected by both methods are significantly correlated, although the correlation is weak (r = 0.32). Thus, in systems with highly duplicated MHC, 454 provides more reliable information on individual diversity than CE-SSCP.

摘要

高度动态的主要组织相容性复合体 (MHC) 的基因与个体适应性直接相关,在进化生态学和保护遗传学中具有重要意义。基因复制和正选择通常会导致 MHC 区域的高水平多态性,使得 MHC 基因分型成为一项具有挑战性的任务。在这里,我们比较了两种用于高度重复 MHC I 基因的雀形目动物 MHC I 基因分型的方法的性能:毛细管电泳-单链构象多态性 (CE-SSCP) 分析和 454 GS FLX Titanium 焦磷酸测序。根据我们的发现,CE-SSCP 检测到的 MHC 变体数量(为简单起见称为等位基因)明显低于 454 检测到的数量。为了解决两种方法之间的差异,我们对一个具有大量等位基因的个体的 MHC I 扩增子进行了克隆和 Sanger 测序。我们发现克隆/Sanger 测序结果与 454 完全一致。因此,在多基因座扩增的情况下,CE-SSCP 大大低估了个体 MHC 的多样性。然而,两种方法检测到的等位基因数量显著相关,尽管相关性较弱(r = 0.32)。因此,在 MHC 高度重复的系统中,454 比 CE-SSCP 提供了更可靠的个体多样性信息。

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