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活化的人B淋巴细胞上II型Fcγ受体表达的调节

Modulation of type II Fc gamma receptor expression on activated human B lymphocytes.

作者信息

Sármay G, Rozsnyay Z, Szabó I, Biró A, Gergely J

机构信息

Department of Immunology, L. Eötvös University, Göd, Hungary.

出版信息

Eur J Immunol. 1991 Mar;21(3):541-9. doi: 10.1002/eji.1830210303.

DOI:10.1002/eji.1830210303
PMID:1826259
Abstract

We have monitored Fc gamma RII expression during the activation of human B lymphocytes by simultaneous analysis of monoclonal antibody (mAb) binding and EA rosetting. The expression of Fc gamma RII showed a biphasic time course. Initially, a transient increase of Fc gamma RII with no ligand-binding capacity was observed with mAb staining as early as 10 min after stimulation by the F(ab')2 fragment of anti-human IgM or phorbol 12-myristate 13-acetate and then after 3 to 24 h a decrease in the number of Fc gamma RII+ cells was seen. Trypsin-like serine protease activity also appeared in the lysate of activated B cells at this time. On the 2nd day of activation a significant enhancement of Fc gamma RII expression was observed, mainly on enlarged blast cells as monitored by both mAb and by ligand binding (EA rosette). At the same time, soluble fragments of Fc gamma RII with the ability to bind human Fc were detected in the supernatant of activated B cells, probably as a result of proteolytic cleavage. These findings suggest that activated B cells are identical with the population of mononuclear cells which shed Fc gamma R when incubated at 37 degrees C. The ability of activated but not resting B cells to release Fc gamma RII correlates with the expression of early activation markers and with the appearance of a trypsin-like serine protease activity of the same cells; thus, the release of Fc gamma RII occurs in the early G1 phase of cell cycle as a result of proteolysis. Later the release of Fc gamma RII is accompanied by the enhancement of Fc gamma RII expression before the cells reach the S phase. The fragments of cleaved Fc gamma RII had an apparent molecular mass of 33 and 14-18 kDa under nonreducing conditions, and upon reduction fragments of smaller size were observed.

摘要

我们通过同时分析单克隆抗体(mAb)结合和EA花环形成,监测了人B淋巴细胞激活过程中FcγRII的表达。FcγRII的表达呈现双相时间进程。最初,早在抗人IgM的F(ab')2片段或佛波醇12-肉豆蔻酸酯13-乙酸酯刺激后10分钟,用mAb染色观察到FcγRII出现短暂增加,但无配体结合能力,然后在3至24小时后,FcγRII+细胞数量减少。此时,活化B细胞裂解物中也出现了类胰蛋白酶丝氨酸蛋白酶活性。在激活的第2天,观察到FcγRII表达显著增强,主要在通过mAb和配体结合(EA花环)监测的增大的母细胞上。同时,在活化B细胞的上清液中检测到具有结合人Fc能力的FcγRII可溶性片段,这可能是蛋白水解裂解的结果。这些发现表明,活化的B细胞与在37℃孵育时脱落FcγR的单核细胞群体相同。活化而非静止的B细胞释放FcγRII的能力与早期激活标志物的表达以及同一细胞类胰蛋白酶丝氨酸蛋白酶活性的出现相关;因此,FcγRII的释放是由于蛋白水解作用在细胞周期的早期G1期发生的。后来,在细胞进入S期之前,FcγRII的释放伴随着FcγRII表达的增强。在非还原条件下,裂解的FcγRII片段的表观分子量为33 kDa和14 - 18 kDa,还原后观察到较小尺寸的片段。

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Modulation of type II Fc gamma receptor expression on activated human B lymphocytes.活化的人B淋巴细胞上II型Fcγ受体表达的调节
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