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通过毛细管电泳检测和鉴定单克隆丙种球蛋白病。

Detection and identification of monoclonal gammopathies by capillary electrophoresis.

作者信息

Henskens Y, de Winter J, Pekelharing M, Ponjee G

机构信息

Klinisch Chemisch Laboratorium, Diagnostisch Centrum SSDZ, Delft, The Netherlands.

出版信息

Clin Chem. 1998 Jun;44(6 Pt 1):1184-90.

PMID:9625041
Abstract

Capillary electrophoresis (CE) and immunosubtraction capillary electrophoresis (IS-CE) were compared with the conventional methods agarose gel electrophoresis (AGE) and immunofixation electrophoresis (IFE) for detection and identification of paraproteins. In total, 74 paraproteins out of 468 serum samples were detected by both methods. Seventy-three monoclonal bands with concentrations ranging from 0.6 to 50.9 g/L were detected by the routine method. With CE, 70 paraproteins were detected and quantified on the electropherogram. Four paraproteins were not detected by CE; three of these were IgG (0.6, 1.1, and 2.2 g/L, respectively), and one was a IgM paraprotein (20.3 g/L) that could be visualized by minor changes in the running conditions. In comparison with IFE, 69 paraproteins were typed identically using IS-CE; only one paraprotein (IgMkappa, 14.9 g/L) could not be identified. On the other hand, a monoclonal IgA band that had not been detected by AGE was identified by CE and IS-CE. We conclude that, in general, CE could be a useful method for detection of paraproteins and that IS-CE is a good alternative to IFE. Additional studies are required to investigate the ionic strength and pH of the running buffer, because these prove to be the most crucial factors for routine CE separation of paraproteins.

摘要

将毛细管电泳(CE)和免疫扣除毛细管电泳(IS-CE)与传统方法琼脂糖凝胶电泳(AGE)和免疫固定电泳(IFE)进行比较,以检测和鉴定副蛋白。总共468份血清样本中的74份副蛋白通过两种方法均被检测到。常规方法检测到73条单克隆条带,浓度范围为0.6至50.9g/L。通过CE,在电泳图上检测并定量了70份副蛋白。CE未检测到4份副蛋白;其中3份是IgG(分别为0.6、1.1和2.2g/L),1份是IgM副蛋白(20.3g/L),通过运行条件的微小变化可使其可视化。与IFE相比,使用IS-CE对69份副蛋白进行了相同分型;仅1份副蛋白(IgMκ,14.9g/L)无法鉴定。另一方面,AGE未检测到的一条单克隆IgA条带通过CE和IS-CE被鉴定出来。我们得出结论,总体而言,CE可能是检测副蛋白的一种有用方法,且IS-CE是IFE的良好替代方法。需要进行更多研究来调查运行缓冲液的离子强度和pH值,因为这些被证明是副蛋白常规CE分离的最关键因素。

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