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利用单克隆抗体对一种非T、非B人类淋巴细胞(L细胞)的特性进行研究。其在B淋巴细胞功能中的调节作用。

Characterization of a non-T, non-B human lymphocyte (L cell) with use of monoclonal antibodies. Its regulatory role in B lymphocyte function.

作者信息

Lobo P I

出版信息

J Clin Invest. 1981 Aug;68(2):431-8. doi: 10.1172/jci110272.

Abstract

These studies investigate the role of L lymphocytes in regulating terminal B lymphocyte differentiation. L cells have abundant Fc IgG receptors and comprise 10--15% of human peripheral blood mononuclear cells (PBMC). L cells lack the conventional markers of B and T lymphocytes and in culture, do not develop into B cells, T cells, or macrophages. Additionally, use of monoclonal antibodies failed to detect on L cells, surface antigens specific for B cells, T cells, and macrophages. In these studies, purified L cell subpopulations depleted of macrophages were co-cultured with autologous PBMC in the presence of pokeweed mitogen and at the end of 8 d, development of intracytoplasmic immunoglobulin (Ig) was determined. L cells were depleted of B and T cells by rosetting techniques and, in addition, by cytotoxicity techniques using monoclonal-specific antisera to T cells. In 14 individuals, L cells when co-cultured with PBMC, enhanced Ig synthesis by 83% +/- 62 SD, and also enhanced cell proliferation. Radiated L cells lost enhancing properties. To study the role of their high density Fc IgG receptors, L cells pretreated with IgG antibody-sensitized erythrocytes were used (i.e., after lysis of rosettes). Such L cells significantly inhibited Ig synthesis (by greater than 50%) despite promoting cell proliferation. Antibody-sensitized erythrocyte-rosetted macrophages did not inhibited Ig synthesis. Thus, positive and negative influences can be mediated by the same cell, depending on the state of Fc-receptor stimulation. Such cells may play a more prominent role in "feed-back" regulation of Ig synthesis by virtue of having abundant Fc IgG receptors.

摘要

这些研究调查了L淋巴细胞在调节终末B淋巴细胞分化中的作用。L细胞有丰富的Fc IgG受体,占人外周血单个核细胞(PBMC)的10% - 15%。L细胞缺乏B和T淋巴细胞的传统标志物,在培养中不会发育成B细胞、T细胞或巨噬细胞。此外,使用单克隆抗体未能在L细胞上检测到B细胞、T细胞和巨噬细胞特有的表面抗原。在这些研究中,去除巨噬细胞的纯化L细胞亚群与自体PBMC在商陆有丝分裂原存在的情况下共培养,在8天结束时,测定胞质内免疫球蛋白(Ig)的发育情况。通过玫瑰花结技术以及使用针对T细胞的单克隆特异性抗血清的细胞毒性技术,使L细胞去除B和T细胞。在14名个体中,L细胞与PBMC共培养时,Ig合成增强了83%±62 SD,并且细胞增殖也增强。经辐射的L细胞失去了增强特性。为了研究其高密度Fc IgG受体的作用,使用了用IgG抗体致敏红细胞预处理的L细胞(即玫瑰花结裂解后)。尽管促进细胞增殖,但这种L细胞显著抑制Ig合成(超过50%)。抗体致敏红细胞玫瑰花结化的巨噬细胞不抑制Ig合成。因此,取决于Fc受体的刺激状态,可以由同一细胞介导正向和负向影响。由于具有丰富的Fc IgG受体,这类细胞可能在Ig合成的“反馈”调节中发挥更突出的作用。

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