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使用全绵羊红细胞 ELISA 评估体内免疫抑制。

Use of whole sheep red blood cells in ELISA to assess immunosuppression in vivo.

机构信息

Tsukuba Safety Assessment Laboratories, Banyu Pharmaceutical Co., Ltd., Tsukuba, Ibaraki, Japan.

出版信息

J Immunotoxicol. 2007 Jan;4(1):77-82. doi: 10.1080/15476910601161691.

DOI:10.1080/15476910601161691
PMID:18958715
Abstract

An enzyme-linked immunosorbent assay (ELISA) using whole sheep red blood cells (SRBC) has been reported as one of the methods for detecting a T-lymphocyte-dependent antibody response. However, it has not been widely used because of SRBC problems such as the weak attachment to ELISA plates, specificity and short-term stability. The objectives of this study were to address these issues and to validate the SRBC-specific antibody response assay. Male Sprague-Dawley rats were bled after 6 days of SRBC immunization. In our new procedure, glutaraldehyde was added before discarding the supernatant of inoculated SRBC suspension to attach SRBC firmly to the plate, while in the original method it was added after discarding. As a result, the attached SRBC was maintained throughout the ELISA procedures. No interference was observed in the titration curve of IgM and IgG antibodies in rats and IgM-antibody in mice when control sera were analyzed to evaluate specificity of this method. The short-term stability of SRBC was overcome by using the different lots of SRBC. They provided antibody titers, which were consistent with those measured using the same lot for immunization. In addition, cyclophosphamide, cyclosporine, prednisolone and methotrexate, well-known immunosuppressive agents, were tested to confirm the applicability of the improved ELISA method to detect the T-lymphocyte-dependent antibody response. All four compounds inhibited the IgM antibody responses dose-dependently. These results demonstrate that the improved whole SRBC-ELISA method provides reproducible and reliable results in the T-lymphocyte-dependent antibody response assay.

摘要

一种使用全绵羊红细胞(SRBC)的酶联免疫吸附测定(ELISA)已被报道为检测 T 淋巴细胞依赖性抗体反应的方法之一。然而,由于 SRBC 存在问题,如与 ELISA 板的弱附着、特异性和短期稳定性,因此并未得到广泛应用。本研究的目的是解决这些问题并验证 SRBC 特异性抗体反应测定。雄性 Sprague-Dawley 大鼠在 SRBC 免疫 6 天后采血。在我们的新程序中,在丢弃接种的 SRBC 悬浮液的上清液之前加入戊二醛,以使 SRBC 牢固地附着在板上,而在原始方法中,在丢弃后加入。结果,附着的 SRBC 在整个 ELISA 过程中得以维持。当分析对照血清以评估该方法的特异性时,在大鼠的 IgM 和 IgG 抗体滴定曲线以及小鼠的 IgM 抗体中未观察到干扰。通过使用不同批次的 SRBC 克服了 SRBC 的短期稳定性。它们提供的抗体滴度与使用相同批次进行免疫接种所测量的滴度一致。此外,还测试了环磷酰胺、环孢素、泼尼松龙和甲氨蝶呤等众所周知的免疫抑制剂,以确认改良的 ELISA 方法在检测 T 淋巴细胞依赖性抗体反应中的适用性。这四种化合物均剂量依赖性地抑制 IgM 抗体反应。这些结果表明,改良的全 SRBC-ELISA 方法在 T 淋巴细胞依赖性抗体反应测定中提供了可重复和可靠的结果。

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