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在检测定义特定特异性的HLA-DR抗体时避免某些系统性陷阱。

Avoidance of certain systematic pitfalls in the detection of HLA-DR antibodies defining find specificities.

作者信息

Müller C, Fink D, Müller G, Wernet P

出版信息

Tissue Antigens. 1980 Sep;16(3):244-53. doi: 10.1111/j.1399-0039.1980.tb00300.x.

DOI:10.1111/j.1399-0039.1980.tb00300.x
PMID:6970429
Abstract

A selective screening program has been established to identify rapidly and effectively the fine specificity of HLA-DR antibodies in pregnancy anti-HLA sera. Following initial HLA-A, B, C screening sera with extra- or multispecific reactions were selected and specifically tested after platelet absorption on isolated B- and T-lymphocyte populations of the serum donor's husband. Identification of the HLA-DR serum. Multispecific anti-DR sera were defined and rendered operationally monospecific by titration. Some critical steps in a reliable assessment of HLA-DR typing reagents could be worked out. Weak HLA-A, B antibodies, B-cell auto- and Lewis antibodies may cause positive reactivity preferentially or even selectively on B lymphocytes. Of particular importance was the hidden presence of HLA-C specific antibodies, since they cannot be absorbed out of stored platelets. In addition they are not readily detectable through screening on typed panel cells. Because of the frequently very high linkage disequilibrium between HLA-B and HLA-C alleles it is difficult to select appropriately dissecting panel cells. The two points demonstrated above gain even more weight when isolated T and B cell populations are used for HLA-DR typing, because HLA-C antibodies preferentially kill B cells. In this fashion contaminating HLA-C antibodies are not only difficult to detect but can mimic the presence of HLA-DR antibodies.

摘要

已经建立了一个选择性筛查程序,以快速、有效地鉴定妊娠抗HLA血清中HLA - DR抗体的精细特异性。在最初对HLA - A、B、C进行筛查后,选择具有额外或多特异性反应的血清,并在血清供体丈夫的分离B淋巴细胞和T淋巴细胞群体上进行血小板吸附后进行特异性检测。HLA - DR血清的鉴定。通过滴定定义多特异性抗DR血清并使其在操作上成为单特异性。可以确定可靠评估HLA - DR分型试剂的一些关键步骤。弱HLA - A、B抗体、B细胞自身抗体和Lewis抗体可能优先甚至选择性地在B淋巴细胞上引起阳性反应。特别重要的是HLA - C特异性抗体的隐性存在,因为它们不能从储存的血小板中被吸收掉。此外,通过对分型板细胞进行筛查也不容易检测到它们。由于HLA - B和HLA - C等位基因之间经常存在非常高的连锁不平衡,因此很难选择合适的分析板细胞。当使用分离的T细胞和B细胞群体进行HLA - DR分型时,上述两点更为重要,因为HLA - C抗体优先杀死B细胞。以这种方式,污染的HLA - C抗体不仅难以检测,而且可以模拟HLA - DR抗体的存在。

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Avoidance of certain systematic pitfalls in the detection of HLA-DR antibodies defining find specificities.在检测定义特定特异性的HLA-DR抗体时避免某些系统性陷阱。
Tissue Antigens. 1980 Sep;16(3):244-53. doi: 10.1111/j.1399-0039.1980.tb00300.x.
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