Golay J, Cusmano G, Introna M
Istituto di Ricerche Farmacologiche Mario Negri, Milano, Italy.
J Immunol. 1992 Jul 1;149(1):300-8.
Although a detailed picture is emerging about the nature of the second messengers involved in B cell activation and proliferation, little is yet known about the intracellular events taking place further downstream. The c-myb proto-oncogene, the structurally related B-myb gene, and c-myc probably code for transcription factors, have been demonstrated to be necessary for the proliferation of hemopoietic cells, and their expression is indeed induced after mitogenic stimulation of T and B lymphocytes. They are therefore likely to be key elements in the regulation of gene expression during proliferation. We have set out to study the regulation of the expression of these two myb genes and of that of c-myc in relation to entry into the different phases of the cell cycle during mitogenic stimulation of resting human B lymphocytes. Resting tonsillar B cells stimulated with the anti-CD20 antibody 1F5 alone are induced to enter the G1 but not the S phase of the cell cycle, whereas co-stimulation with the anti-CD40 antibody G28.5 further drives them to enter the S phase and proliferate. The G28.5 antibody alone has been reported to partially activate and increase the alertness of resting B cells without inducing them to enter G1. In this report we show that increasing the strength of the activating signal leads to progressive induction of the proliferation-related genes studied. Thus the G28.5 antibody alone induces c-myc mRNA only in resting B cells, 1F5 induces both c-myc and B-myb, and the full mitogenic signal given by both antibodies together is accompanied by increased expression of all three--c-myc, B-myb, and c-myb genes. In addition, using a semi-quantitative polymerase chain reaction method, we show that different inhibitors of B cell proliferation, namely, cyclosporin A, an anti-CD19 antibody (HD37), and transforming growth factor beta 1 (TGF-beta 1), inhibit differentially the induction of these same genes after mitogenic stimulation of B cells. Whereas cyclosporin A inhibits induction of all three genes, TGF-beta 1 specifically blocks B-myb induction and CD19 has little effect on either of the genes tested. We conclude that c-myb, B-myb, and c-myc are regulated independently from one another, that induction of c-myc and B-myb together is not sufficient to trigger B cell proliferation, and we suggest that expression of all three is a prerequisite for proliferation to occur.
尽管有关参与B细胞激活和增殖的第二信使的性质,一幅详细的图景正在浮现,但对于更下游发生的细胞内事件却知之甚少。c-myb原癌基因、结构相关的B-myb基因以及c-myc可能编码转录因子,已被证明是造血细胞增殖所必需的,并且它们的表达确实在T和B淋巴细胞受到促有丝分裂刺激后被诱导。因此,它们很可能是增殖过程中基因表达调控的关键元件。我们着手研究在静止的人B淋巴细胞受到促有丝分裂刺激期间,这两个myb基因以及c-myc基因的表达调控与进入细胞周期不同阶段的关系。单独用抗CD20抗体1F5刺激静止的扁桃体B细胞,可诱导其进入细胞周期的G1期,但不能进入S期,而用抗CD40抗体G28.5共同刺激则进一步促使它们进入S期并增殖。据报道,单独的G28.5抗体可部分激活静止B细胞并提高其警觉性,但不会诱导它们进入G1期。在本报告中,我们表明增强激活信号的强度会导致所研究的增殖相关基因的逐步诱导。因此,单独的G28.5抗体仅在静止B细胞中诱导c-myc mRNA,1F5诱导c-myc和B-myb,而两种抗体共同给出的完整促有丝分裂信号伴随着所有三个基因——c-myc、B-myb和c-myb基因表达的增加。此外,使用半定量聚合酶链反应方法,我们表明B细胞增殖的不同抑制剂,即环孢素A、抗CD19抗体(HD37)和转化生长因子β1(TGF-β1),在B细胞受到促有丝分裂刺激后对这些相同基因的诱导有不同程度的抑制作用。环孢素A抑制所有三个基因的诱导,而TGF-β1特异性阻断B-myb的诱导,CD19对所测试的任何一个基因几乎没有影响。我们得出结论,c-myb、B-myb和c-myc彼此独立调控,c-myc和B-myb的共同诱导不足以触发B细胞增殖,并且我们认为所有三个基因的表达是增殖发生的先决条件。
