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小鼠IgG结合因子(IgG-BF)的大小和电荷异质性

Size and charge heterogeneity of murine IgG-binding factors (IgG-BF).

作者信息

Blank U, Fridman W H, Daëron M, Galinha A, Moncuit J, Néauport-Sautès C

出版信息

J Immunol. 1986 Apr 15;136(8):2975-82.

PMID:3514751
Abstract

Size and charge of murine IgG-binding factors (IgG-BF) were determined. Four different sources were used to produce the factors: a) cells of a T cell hybrid (T2D4) constitutively secreting IgG-BF upon incubation in serum-free medium, b) T2D4 cells incubated with mouse monoclonal IgG1 antibody in order to induce in vitro the production of isotype-specific IgG1-BF, c) T2D4 cells induced in vivo by passage as ascites in nude mice and incubated in serum-free medium, and d) in vivo alloantigen-activated T cells (ATC) incubated in serum-free medium. IgG-BF were affinity purified on Sepharose beads coated with rabbit or mouse IgG and identified by their biologic activities, i.e., inhibition of in vitro secondary IgG antibody production to SRBC and inhibition of rosette formation between Fc gamma receptor-positive spleen cells and rabbit IgG-sensitized erythrocytes. IgG-BF produced by either of these cell sources was found to be heterogeneous in both size and charge. In each case, IgG-BF activities were recovered in three fractions of apparent Mr-74,000 to 78,000, 35,000 to 40,000, and 19,000 to 23,000-and in four fractions of pI-4.7 (or 5.3, depending on experimental conditions), 6.5, 7.7, and 8.4. Moreover, IgG-BF translated in vitro from T2D4 poly A RNA by using rabbit reticulocyte lysate exhibited the same heterogeneity. Thus, IgG-BF contain different proteins exerting similar biologic activities.

摘要

测定了小鼠IgG结合因子(IgG-BF)的大小和电荷。使用了四种不同来源来产生这些因子:a)一种T细胞杂交体(T2D4)的细胞,在无血清培养基中孵育时可组成性分泌IgG-BF;b)将T2D4细胞与小鼠单克隆IgG1抗体一起孵育,以体外诱导产生同种型特异性IgG1-BF;c)通过在裸鼠体内传代形成腹水而在体内诱导的T2D4细胞,并在无血清培养基中孵育;d)在无血清培养基中孵育的体内同种异体抗原激活的T细胞(ATC)。IgG-BF在包被有兔或小鼠IgG的琼脂糖珠上进行亲和纯化,并通过其生物学活性进行鉴定,即抑制体外针对SRBC的二级IgG抗体产生以及抑制Fcγ受体阳性脾细胞与兔IgG致敏红细胞之间的玫瑰花结形成。发现由这些细胞来源中的任何一种产生的IgG-BF在大小和电荷上均具有异质性。在每种情况下,IgG-BF活性在三个表观Mr为74,000至78,000、35,000至40,000以及19,000至23,000的组分中回收,并且在四个pI为4.7(或5.3,取决于实验条件)、6.5、7.7和8.4的组分中回收。此外,使用兔网织红细胞裂解物从T2D4多聚A RNA体外翻译的IgG-BF表现出相同的异质性。因此,IgG-BF包含发挥相似生物学活性的不同蛋白质。

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