Long-range PCR amplification as an alternative strategy for characterizing novel HLA-B alleles

被引:32
作者
Curran, MD
Williams, F
Earle, JAP
Rima, BK
vanDam, MG
Bunce, M
Middleton, D
机构
[1] QUEENS UNIV BELFAST,SCH BIOL & BIOCHEM,BELFAST,ANTRIM,NORTH IRELAND
[2] ST MARYS HOSP,TISSUE TYPING TRANSPLANT UNIT,LONDON,ENGLAND
[3] CHURCHILL HOSP,TISSUE TYPING LAB,OXFORD TRANSPLANT CTR,OXFORD OX3 7LJ,ENGLAND
来源
EUROPEAN JOURNAL OF IMMUNOGENETICS | 1996年 / 23卷 / 04期
关键词
D O I
10.1111/j.1744-313X.1996.tb00125.x
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
We have developed a simple, rapid and reliable method for specifically amplifying and cloning full-length HLA-B genes from genomic DNA. Using this methodology we characterized three alleles of interest at the molecular level. Two of the alleles appeared in our routine class I PCR-SSOP typing system, a variant of B*5801 found in the Daudi cell line and RCE 56 and a variant of B*4101 found in a number of volunteer donors on our Bone Marrow Donor Registry. The third, a variant B35 allele found in RCE 80, was first identified as unusual by serology. Our sequencing analysis of exon 2 and exon 3 identified two of these alleles as the recently reported novel HLA-B*5802 and HLA-B*4102 alleles, while the third represents a new B35 allele officially designated B*3513.
引用
收藏
页码:297 / 309
页数:13
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