中华医学遗传学杂志
中華醫學遺傳學雜誌
중화의학유전학잡지
CHINESE JOURNAL OF MEDICAL GENETICS
2009年
5期
562-566
,共5页
曾健强%徐筠娉%王大明%邹红岩%邓志辉%杨宝成
曾健彊%徐筠娉%王大明%鄒紅巖%鄧誌輝%楊寶成
증건강%서균빙%왕대명%추홍암%산지휘%양보성
人类白细胞抗原%HLA-C基因%测序分型%克隆%测序分析%等位基因丢失
人類白細胞抗原%HLA-C基因%測序分型%剋隆%測序分析%等位基因丟失
인류백세포항원%HLA-C기인%측서분형%극륭%측서분석%등위기인주실
human leukocyte antigen%HLA-C gene%sequence-based typing%cloning%sequencing analysis%allele dropout
目的 探讨HLA-C基因测序分型时等位基因漏检和丢失的原因,以提高HLA测序分型的成功率和准确性.方法 620份随机选择的深圳健康捐血者血样,采用AlleleSEQR HLA-C plus测序分型试剂盒进行检测,对无完全匹配、分型结果"异常"的标本,采用分子克隆和测序方法进行全长单倍体序列分析;对未检出新的碱基点突变的样本,进一步采用自行设计的PCR引物和AlleleSEQR试剂盒中的测序引物进行再测序,分析测序分型结果"异常"的原因.结果 620份经AlleleSEQR HLA-C测序分型的样本中,发现5例样本无完全匹配的基因型,与之最接近的多种等位基因型均存在单个碱基的不匹配;并且在第4外显子出现碱基杂合,但第2和第3外显子区域内无杂合碱基.经分子克隆和单倍体测序,以及采用自行设计的PCR引物和AlleleSEQR试剂盒中的测序引物再测序,证实了5例标本均存在Cw * 0706等位基因漏检和丢失现象,未发现新的碱基点突变.结论 HLA-C基因测序分型时,因PCR引物与模板DNA不匹配会导致等位基因的漏检和丢失.根据中国人群HLA-C分子全长序列特点,开发适合于中国人群的测序分型试剂十分必要.
目的 探討HLA-C基因測序分型時等位基因漏檢和丟失的原因,以提高HLA測序分型的成功率和準確性.方法 620份隨機選擇的深圳健康捐血者血樣,採用AlleleSEQR HLA-C plus測序分型試劑盒進行檢測,對無完全匹配、分型結果"異常"的標本,採用分子剋隆和測序方法進行全長單倍體序列分析;對未檢齣新的堿基點突變的樣本,進一步採用自行設計的PCR引物和AlleleSEQR試劑盒中的測序引物進行再測序,分析測序分型結果"異常"的原因.結果 620份經AlleleSEQR HLA-C測序分型的樣本中,髮現5例樣本無完全匹配的基因型,與之最接近的多種等位基因型均存在單箇堿基的不匹配;併且在第4外顯子齣現堿基雜閤,但第2和第3外顯子區域內無雜閤堿基.經分子剋隆和單倍體測序,以及採用自行設計的PCR引物和AlleleSEQR試劑盒中的測序引物再測序,證實瞭5例標本均存在Cw * 0706等位基因漏檢和丟失現象,未髮現新的堿基點突變.結論 HLA-C基因測序分型時,因PCR引物與模闆DNA不匹配會導緻等位基因的漏檢和丟失.根據中國人群HLA-C分子全長序列特點,開髮適閤于中國人群的測序分型試劑十分必要.
목적 탐토HLA-C기인측서분형시등위기인루검화주실적원인,이제고HLA측서분형적성공솔화준학성.방법 620빈수궤선택적심수건강연혈자혈양,채용AlleleSEQR HLA-C plus측서분형시제합진행검측,대무완전필배、분형결과"이상"적표본,채용분자극륭화측서방법진행전장단배체서렬분석;대미검출신적감기점돌변적양본,진일보채용자행설계적PCR인물화AlleleSEQR시제합중적측서인물진행재측서,분석측서분형결과"이상"적원인.결과 620빈경AlleleSEQR HLA-C측서분형적양본중,발현5례양본무완전필배적기인형,여지최접근적다충등위기인형균존재단개감기적불필배;병차재제4외현자출현감기잡합,단제2화제3외현자구역내무잡합감기.경분자극륭화단배체측서,이급채용자행설계적PCR인물화AlleleSEQR시제합중적측서인물재측서,증실료5례표본균존재Cw * 0706등위기인루검화주실현상,미발현신적감기점돌변.결론 HLA-C기인측서분형시,인PCR인물여모판DNA불필배회도치등위기인적루검화주실.근거중국인군HLA-C분자전장서렬특점,개발괄합우중국인군적측서분형시제십분필요.
Objective To analyze the possible reason for HLA-C allele dropout in routine sequence-based typing (SBT) and improve the accuracy of HLA-C SBT test. Methods A total of 620 randomly selected samples from healthy voluntary blood donors in Shenzhen were typed at HLA-C locus by sequence-based typing using the AlleleSEQR HLA-C plus sequence-based typing kit. Samples with no full match result were subjected to cloning and haplotype sequencing of the full-length HLA-C gene. If no novel mutations were found, samples were then retyped, using our self-designed PCR primer pair and PCR conditions replacing the AlleleSEQR HLA-C PCR reagents in the PCR set-up procedure so as to analyze the potential reasons t'or causing "abnormal" SBT result. Results In the 620 samples typed at HLA-C locus using the AlleleSEQR HLA-C SBT commercial kit, 5 samples with no full match result were identified. The closest genotype showed one nucleotide mismatch with many different allele groups at different nucleotide position. Based on the PCR-SBT nucleotide sequence, heterozygous nucleotides were determined only in exon 4, whereas the nucleotides in exon 2 and 3 were all homozygotes. The results showed that HLA-Cw * 0706 allele dropout existed in all the 5 samples with "abnormal" SBT results initially identified by AlleleSEQR HLA-C SBT kit, no novel mutation was found. Conclusion The results indicate that the PCR primer pair incompatible with DNA template may result in allele dropout in HLA-C SBT test. Based on the characterization of HLA-C full-length, it is essential to develop HLA-C SBT kit suitable for Chinese population in the future.
