Rosti V, Bergamaschi G, Lucotti C, Danova M, Carlo-Stella C, Locatelli F, Tonon L, Mazzini G, Cazzola M
Department of Internal Medicine, University of Pavia, Italy.
Blood. 1995 Nov 1;86(9):3387-93.
A number of experimental observations suggest that the proto-oncogene c-abl participates in the regulation of hematopoietic cell growth. We used an antisense strategy to study the relationship between c-abl expression and hematopoietic cell proliferation and differentiation. Purified normal human bone marrow-derived CD34+ cells were obtained by immunomagnetic selection and incubated with 18-base-unmodified antisense oligodeoxynucleotides complementary to the first six codons of the two alternative first exons of c-abl, la and lb. At the end of incubation, an aliquot of cells was assayed for clonogenic growth and the remainder was used for flow cytometric analyses. Cell kinetics were evaluated by means of both single parameter DNA and bivariate DNA/bromodeoxyuridine (BrdU) flow cytometry. Apoptosis was routinely studied by DNA flow cytometric analysis and, in some cases, also through DNA agarose gel electrophoresis for detection of oligonucleosomal DNA fragments. Expression of differentiation markers was studied by flow cytometry. Exposure to antisense oligonucleotides specifically inhibited the accumulation of c-abl mRNA in CD34+ cells. Preincubation with the c-abl antisense oligomers reduced the proportion of cells in S-phase from 19% +/- 5% (mean +/- SD) to 7% +/- 4% (P < .05), and BrdU labeling from 13% +/- 6% to 6% +/- 3% (P < .05). Flow cytometry and DNA agarose gel electrophoresis showed that treated CD34+ cells accumulated in the G0/G1 region of the DNA histogram with no evidence of either differentiation or apoptosis. By contrast, both growth factor deprivation and exposure of CD34+ cells to the tyrosine kinase inhibitor tyrphostin AG82 clearly induced apoptosis. When cells were preincubated with antisense oligonucleotides and then plated for evaluation of colony formation, this resulted in a significant inhibition of colony forming unit granulocyte-macrophage growth (from 44 +/- 15 to 22 +/- 9; P < .01) but had no effect on burst-forming unit erythroid growth (24 +/- 11 v 21 +/- 11; P < .05). These results suggest that c-abl expression is critical for entry of human CD34+ hematopoietic cells into S-phase and for their differentiation to granulocyte-macrophage progenitors. They also indicate that other tyrosine kinases besides p145c-alb are active in the prevention of apoptosis, so that inhibition of c-abl RNA accumulation arrests CD34+ cells in G0/G1 without activating programmed death.
多项实验观察结果表明,原癌基因c-abl参与造血细胞生长的调节。我们采用反义策略来研究c-abl表达与造血细胞增殖及分化之间的关系。通过免疫磁珠分选获得纯化的正常人骨髓来源的CD34+细胞,并将其与18个碱基未修饰的反义寡脱氧核苷酸一起孵育,该反义寡脱氧核苷酸与c-abl的两个可变第一外显子la和lb的前六个密码子互补。孵育结束时,取一部分细胞检测集落形成生长情况,其余细胞用于流式细胞术分析。通过单参数DNA和双变量DNA/溴脱氧尿苷(BrdU)流式细胞术评估细胞动力学。通过DNA流式细胞术常规研究细胞凋亡,在某些情况下,也通过DNA琼脂糖凝胶电泳检测寡核小体DNA片段来研究细胞凋亡。通过流式细胞术研究分化标志物的表达。暴露于反义寡核苷酸可特异性抑制CD34+细胞中c-abl mRNA的积累。用c-abl反义寡聚物预孵育可使处于S期的细胞比例从19%±5%(平均值±标准差)降至7%±4%(P<.05),BrdU标记率从13%±6%降至6%±3%(P<.05)。流式细胞术和DNA琼脂糖凝胶电泳显示,经处理的CD34+细胞在DNA直方图的G0/G1区域积累,没有分化或凋亡的迹象。相比之下,生长因子剥夺和CD34+细胞暴露于酪氨酸激酶抑制剂 tyrphostin AG82均明显诱导细胞凋亡。当细胞用反义寡核苷酸预孵育,然后接种以评估集落形成时,这导致集落形成单位粒细胞-巨噬细胞生长受到显著抑制(从44±15降至22±9;P<.01),但对红系爆式集落形成单位生长没有影响(24±11对21±11;P<.05)。这些结果表明,c-abl表达对于人CD34+造血细胞进入S期及其向粒细胞-巨噬细胞祖细胞的分化至关重要。它们还表明,除了p145c-alb之外的其他酪氨酸激酶在预防细胞凋亡中起作用,因此抑制c-abl RNA积累可使CD34+细胞停滞在G0/G1期而不激活程序性死亡。
