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食蟹猴(Macaca fascicularis)和恒河猴(M. mulatta)ABO 基因座外显子 7 的部分序列分析:表现为不定血型表型的个体存在 O 血型。

Partial sequence analyses of exon 7 of the ABO locus of cynomolgus (Macaca fascicularis) and rhesus (M. mulatta) macaques: Indeterminate phenotypes show the presence of the O blood group.

机构信息

School of Mathematical and Natural Sciences, Arizona State University (ASU) at the West Campus, Glendale, Arizona.

California National Primate Research Center, University of California, Davis, California.

出版信息

HLA. 2019 Dec;94(6):482-492. doi: 10.1111/tan.13675. Epub 2019 Sep 3.

DOI:10.1111/tan.13675
PMID:31448567
Abstract

Compatibility tests to identify A, B, and O alleles are critical for establishing suitable donor-recipient matches among experimental animals. Using a qPCR-based SNP probe assay, we have identified A, B, AB, and indeterminate blood group phenotypes in cynomolgus and rhesus macaques. We have hypothesized, albeit without molecular confirmation, that the indeterminate phenotype represents homozygosity for the null O allele at the macaque ABO locus. The indeterminate phenotype represents the unsuccessful detection of either A or B alleles using primers targeting the A-specific and B-specific single nucleotide polymorphisms (SNPs) in a variable region of exon 7 of the ABO locus. These SNPs are associated with two functional sites, detected using two allele-specific probes in the qPCR assay where the codons leucine and methionine (at codon 266) and glycine and alanine (at codon 268) are required for the synthesis of the A and B transferases, respectively. While reference sequences for the A and B alleles exhibited no novel mutations in the functional exon, plasmid Sanger sequence analyses showed unique mutations within the diagnostic target sites in 10 macaques exhibiting the indeterminate phenotype. Eight of these indeterminate individuals exhibited SNPs at codon 268 that should prevent the syntheses of an A or B transferase. While the two other indeterminate samples had functional codons that were consistent with A or B alleles, mutations in either their probe- or primer-binding sites that altered their peptide sequences probably impeded their detection by our assay.

摘要

为了在实验动物中建立合适的供体-受体匹配,对 A、B 和 O 等位基因进行兼容性测试至关重要。我们使用基于 qPCR 的 SNP 探针检测法,鉴定了食蟹猴和恒河猴的 A、B、AB 和不定血型表型。我们假设,尽管没有分子确认,不定血型表型代表在 ABO 基因座上对 null O 等位基因的纯合性。不定血型表型代表使用针对 ABO 基因座 7 号外显子可变区中的 A 特异性和 B 特异性单核苷酸多态性(SNP)的引物未能检测到 A 或 B 等位基因。这些 SNP 与两个功能位点相关,使用 qPCR 检测中的两个等位基因特异性探针检测到,其中编码亮氨酸和蛋氨酸(在密码子 266)和甘氨酸和丙氨酸(在密码子 268)的密码子分别是合成 A 和 B 转移酶所必需的。虽然 A 和 B 等位基因的参考序列在功能外显子中没有新的突变,但质粒 Sanger 序列分析显示在 10 只表现出不定血型表型的猕猴中,在诊断靶位有独特的突变。在这 8 只不定血型个体中,有 268 密码子的 SNP 应该阻止 A 或 B 转移酶的合成。而另外两个不定血型样本具有与 A 或 B 等位基因一致的功能密码子,但它们的探针或引物结合位点的突变改变了它们的肽序列,可能会阻碍我们的检测。

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