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新型多重 PCR-SSP 方法用于着丝粒 KIR 等位基因的区分。

Novel multiplex PCR-SSP method for centromeric KIR allele discrimination.

机构信息

Immunology Program, Sloan-Kettering Institute for Cancer Research, New York, NY, USA.

Department of Pediatrics, Memorial Sloan Kettering Cancer Center, New York, NY, USA.

出版信息

Sci Rep. 2018 Oct 5;8(1):14853. doi: 10.1038/s41598-018-33135-1.

Abstract

Allelic diversity of the KIR2DL receptors drive differential expression and ligand-binding affinities that impact natural killer cell function and patient outcomes for diverse cancers. We have developed a global intermediate resolution amplification-refractory mutation system (ARMS) PCR-SSP method for distinguishing functionally relevant subgroups of the KIR2DL receptors, as defined by phylogenetic study of the protein sequences. Use of the ARMS design makes the method reliable and usable as a kit, with all reactions utilizing the same conditions. Six reactions define six subgroups of KIR2DL1; four reactions define three subgroups of KIR2DL2; and five reactions define four subgroups of KIR2DL3. Using KIR allele data from a cohort of 426 European-Americans, we identified the most common KIR2DL subtypes and developed the high-throughput PCR-based methodology, which was validated on a separate cohort of 260 healthy donors. Linkage disequilibrium analysis between the different KIR2DL alleles revealed that seven allelic combinations represent more than 95% of the observed population genotypes for KIR2DL1/L2/L3. In summary, our findings enable rapid typing of the most common KIR2DL receptor subtypes, allowing more accurate prediction of co-inheritance and providing a useful tool for the discrimination of observed differences in surface expression and effector function among NK cells exhibiting disparate KIR2DL allotypes.

摘要

KIR2DL 受体的等位基因多样性驱动了不同的表达和配体结合亲和力,从而影响自然杀伤细胞的功能和多种癌症患者的预后。我们开发了一种全球中等分辨率扩增-耐药突变系统(ARMS)PCR-SSP 方法,用于区分 KIR2DL 受体的功能相关亚群,该方法是通过对蛋白质序列的系统发育研究来定义的。ARMS 设计的使用使该方法可靠且可作为试剂盒使用,所有反应都利用相同的条件。六个反应定义了 KIR2DL1 的六个亚群;四个反应定义了 KIR2DL2 的三个亚群;五个反应定义了 KIR2DL3 的四个亚群。使用来自 426 名欧洲裔美国人队列的 KIR 等位基因数据,我们确定了最常见的 KIR2DL 亚型,并开发了高通量基于 PCR 的方法,该方法在另外 260 名健康供体的队列中得到了验证。不同 KIR2DL 等位基因之间的连锁不平衡分析表明,七种等位基因组合代表了 KIR2DL1/L2/L3 观察到的人群基因型的 95%以上。总之,我们的研究结果能够快速对最常见的 KIR2DL 受体亚型进行分型,从而更准确地预测共同遗传,并为区分具有不同 KIR2DL 同种型的 NK 细胞表面表达和效应功能的观察到的差异提供有用的工具。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e8a1/6173694/d41a7df4fa5f/41598_2018_33135_Fig1_HTML.jpg

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