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从正常小鼠血清中分离免疫球蛋白E(IgE)

Isolation of IgE from normal mouse serum.

作者信息

Lehrer S B

出版信息

Immunology. 1979 Jan;36(1):103-9.

Abstract

Mouse IgE was isolated from reaginic ascitic fluid and an antiserum to it was produced in rabbits. An immunoadsorbent, prepared with this antiserum, was used to isolate IgE from normal mouse serum. Mouse serum proteins, isolated by (NH4)2SO4 (40--60%) precipitation, were applied to the anti-IgE immunoadsorbent and eluted with 3 M KI or 3.5 M NaSCN. In addition to containing IgE, the eluate contained other immunoglobulins which were subsequently removed with specific immunoadsorbents to IgG1, IgG2a, IgG2b, IgA and IgM. Further purification was achieved by gel filtration on Bio Gel A 0.5 m, ion exchange chromatography on DEAE cellulose, and Pevikon block electrophoresis. Since non-immunoglobulin components were demonstrated by immunoelectrophoresis, IgE was isolated from this pool with an anti-Fab immunoadsorbent and eluted with 3.5 M NaSCN. Based on recovery of 987 micrograms IgE from 855 ml NMS, IgE concentration was estimated at 1.15 microgram/ml. Analysis of purified IgE by immunoelectrophoresis and immunoprecipitation in gel detected a single component, partially identical to isoelectric focused rat IgE myelomas IR162 and IR331 Antiserum to it could completely abolish 48 h but not 2 h passive cutaneous anaphylaxis (PCA) reactions. Normal IgE, when used as a diluent, could inhibit 48 h PCA reaction of reaginic antibody suggesting that it binds to mouse skin in a way similar to reagin. This demonstrates that IgE can be isolated from normal mouse serum. The availability of this source of mouse IgE should facilitate further use of this animal model in studies of allergic reactions.

摘要

从小鼠反应素性腹水液中分离出小鼠IgE,并在兔体内制备了针对它的抗血清。用该抗血清制备的免疫吸附剂用于从正常小鼠血清中分离IgE。通过硫酸铵(40 - 60%)沉淀分离得到的小鼠血清蛋白,应用于抗IgE免疫吸附剂,并用3M KI或3.5M NaSCN洗脱。洗脱液中除了含有IgE外,还含有其他免疫球蛋白,随后用针对IgG1、IgG2a、IgG2b、IgA和IgM的特异性免疫吸附剂将其去除。通过在Bio Gel A 0.5m上进行凝胶过滤、在DEAE纤维素上进行离子交换色谱以及Pevikon块电泳实现了进一步纯化。由于免疫电泳显示存在非免疫球蛋白成分,用抗Fab免疫吸附剂从该组分中分离出IgE,并用3.5M NaSCN洗脱。基于从855ml正常小鼠血清中回收987微克IgE,估计IgE浓度为1.15微克/毫升。通过免疫电泳和凝胶免疫沉淀分析纯化的IgE,检测到单一成分,与等电聚焦大鼠IgE骨髓瘤IR162和IR331部分相同。针对它的抗血清可以完全消除48小时但不能消除2小时的被动皮肤过敏反应(PCA)。正常IgE用作稀释剂时,可以抑制反应素性抗体的48小时PCA反应,表明它以与反应素类似的方式与小鼠皮肤结合。这表明可以从正常小鼠血清中分离出IgE。这种小鼠IgE来源的可得性应有助于在过敏反应研究中进一步利用这种动物模型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/36e5/1457396/d8fcb90ba5e0/immunology00266-0111-a.jpg

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