• 分别设计MSX1PAX9基因特异性引物,聚合酶链反应扩增全部编码内含子-外显子剪接序列,产纯化后直接测序。

    Specific primers were designed for MSX1 and PAX9 respectively. Mutation analysis was performed by direct sequencing of all the coding exons and intron-exon boundaries.

    youdao

  • 研究通过设计合成hla基因序列特异性引物,建立了HLA -DR基因分型的套式扩增直接扩增pcr -SSP技术,骨髓移植配型中进行了应用。

    In this study, a nested PCR SSP and a direct amplification PCR SSP protocols for HLA DR genotyping were developed and were used in the selection of matched donor for sibling BMT.

    youdao

  • 方法设计出针对各片段的特异性引物P CR方法Z 37病毒感染细胞提取细胞rna逆转录扩增克隆t载体,纯化后测序,测定的序列应用DNASTAR软件比较分析。

    Methods the total RNA was extracted from Z37 virus infected cells and the RT-PCR products were cloned into t vector, sequenced and analyzed by DNASTAR software.

    youdao

  • 然后分别提取84例拟进行造血干细胞移植病人及家系成员的外周血d NA,采用RSCA序列特异性引物体外基因扩增(PCRssp)法平行对照对HLA A基因位点进行分

    DNA samples of related hematopoietic stem cell transplant donor-recipients were extracted from peripheral blood cells. HLA-A loci were typed both by RSCA and PCR-SSP.

    youdao

  • 然后分别提取84例拟进行造血干细胞移植病人及家系成员的外周血d NA,采用RSCA序列特异性引物体外基因扩增(PCRssp)法平行对照对HLA A基因位点进行分

    DNA samples of related hematopoietic stem cell transplant donor-recipients were extracted from peripheral blood cells. HLA-A loci were typed both by RSCA and PCR-SSP.

    youdao

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