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通过化学发光分析灵敏检测小鼠巨噬细胞的两种IgG Fc受体

Sensitive detection of two IgG Fc receptors of mouse macrophages by chemiluminescence analysis.

作者信息

Majima T, Itoh K, Yatsu J, Yoshie O, Ishida N

机构信息

Department of Bacteriology, Tohoku University School of Medicine, Sendai.

出版信息

Immunopharmacol Immunotoxicol. 1989;11(2-3):289-307. doi: 10.3109/08923978909005371.

Abstract

Luminol-enhanced chemiluminescence assay was used to detect the surface expression and the consequent activation of receptors (FcRI and FcRII) of murine macrophages (M phi s). When murine IgG2a was used for the specific detection of FcRI and IgG2b for FcRII, a newly established procedure enabled us to detect the activation of each receptor with as few as 3 X 10(5) M phi s. Briefly, TNP-SRBC coated with monoclonal IgG2a or IgG2b antibodies directed to TNP (sensitized SRBC) were used as reagent, in the presence of 1 X 10(-5) M luminol, and the emission was measured with a liquid scintillation counter. When results obtained by chemiluminescence counting were compared to the results obtained by the rosette formation by adding the same SRBC reagent to peritoneal M phi s obtained after ip injection of Listeria, fortified chemiluminescence counting allowed us to obtain a more definite answer about the activation of each receptor. Under the conditions established, the specific activation of FcRI was obtained by the addition of rIFN alpha A/D to the resident M phi s in vitro and the specific activation of spleen M phi FcRII by iv injection of IAP (Immunosuppressive acidic protein) into mice. These two results supported the independence of the two receptors detected by the assay.

摘要

采用鲁米诺增强化学发光分析法检测小鼠巨噬细胞(M phi s)表面受体(FcRI和FcRII)的表达及其激活情况。当用鼠IgG2a特异性检测FcRI,用IgG2b检测FcRII时,一种新建立的方法使我们能够用低至3×10⁵个M phi s检测每种受体的激活情况。简要地说,用包被有针对TNP的单克隆IgG2a或IgG2b抗体的TNP - SRBC(致敏SRBC)作为试剂,在存在1×10⁻⁵ M鲁米诺的情况下,用液体闪烁计数器测量发光。当将化学发光计数得到的结果与通过向腹腔注射李斯特菌后获得的腹腔M phi s中加入相同的SRBC试剂形成花环得到的结果进行比较时,强化化学发光计数使我们能够对每种受体的激活情况获得更明确的答案。在既定条件下,通过在体外向驻留M phi s中添加rIFNαA/D获得FcRI的特异性激活,通过向小鼠静脉注射IAP(免疫抑制酸性蛋白)获得脾M phi FcRII的特异性激活。这两个结果支持了该分析方法检测到的两种受体的独立性。

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