Podo F, Ferretti A, Knijn A, Zhang P, Ramoni C, Barletta B, Pini C, Baccarini S, Pulciani S
Department of Cell Biology, Istituto Superiore di Sanità, Roma, Italy.
Anticancer Res. 1996 May-Jun;16(3B):1399-412.
Although evidence supports constitutive activation of phosphatidylcholine specific phospholipase C (PC-plc) in rastransformed fibroblasts, no studies have been devoted to measure the basal activity levels of this enzyme, its molecular characteristics and subcellular localization. This paper reports for the first time measurements of the activity of different enzymes responsible for PC hydrolysis (PC-plc; phospholipases A2 (pla2) and A1 (pla1)) in homogenates of murine NIH-3T3 fibroblasts (3T3) and their transformants obtained by human H-ras transfection (3T3ras). To this end, 31P NMR analyses were carried out on total cell homogenates, incubated in the presence of mixed diheptanoylphosphatidylcholine: sphingomyelin (DHPC:SM) unilamellar vesicles (SLUV), in which DHPC acts as a suitable substrate for water-soluble lipolytic enzymes. The basal PC-plc activity levels (0.66 +/- 0.14 and 0.38 +/- 0.10 nmol/10(6) cells.hour in 3T3 and 3T3ras fibroblasts, respectively),were substantially higher (over 30-50x) than those reported in the literature for normal mammalian cells (dog heart myocytes). Moreover the PC-plc activity was about 15-30 times lower than the overall PC deacylation activity in both clones. The use of high titer polyclonal antibodies, raised in a rabbit against bacterial PC-plc, allowed identification of one cross-reactive mammalian PC-plc component (M(r) 66 kD) in cell lysates of both 3T3 and 3T3ras fibroblasts, and detection, by indirect immunofluorescence, of its subcellular localization. In control 3T3 fibroblasts (in the late log-phase of growth) the enzyme was exclusively located in the cytosol, while in H-ras transformed cells it was massively exposed on the external side of the membrane. This new finding strongly suggests that the oncogenic product p2Iras is able to induce (or mediate) translocation of PC-plc across the plasma membrane of ras transformed cells, with possible implications not only on cell biochemistry (enhancement of PC-plc activity, and consequent production of intra- and extracellular PCho and accumulation of neutral lipids) but also on cell-cell interaction mechanisms which facilitate tumour invasion and metastasis of oncogene-transformed cells.
尽管有证据支持磷脂酰胆碱特异性磷脂酶C(PC - plc)在ras转化的成纤维细胞中组成性激活,但尚未有研究致力于测量该酶的基础活性水平、其分子特征和亚细胞定位。本文首次报道了在小鼠NIH - 3T3成纤维细胞(3T3)及其通过人H - ras转染获得的转化体(3T3ras)的匀浆中,对负责PC水解的不同酶(PC - plc;磷脂酶A2(pla2)和A1(pla1))活性的测量。为此,对在混合二庚酰磷脂酰胆碱:鞘磷脂(DHPC:SM)单层囊泡(SLUV)存在下孵育的全细胞匀浆进行了31P NMR分析,其中DHPC作为水溶性脂解酶的合适底物。基础PC - plc活性水平(在3T3和3T3ras成纤维细胞中分别为0.66±0.14和0.38±0.10 nmol/10(6)细胞·小时),比文献报道的正常哺乳动物细胞(犬心肌细胞)的活性水平高得多(超过30 - 50倍)。此外,在两个克隆中,PC - plc活性比总的PC脱酰基活性低约15 - 30倍。使用在兔体内针对细菌PC - plc产生的高滴度多克隆抗体,能够在3T3和3T3ras成纤维细胞的细胞裂解物中鉴定出一种交叉反应的哺乳动物PC - plc成分(分子量66 kD),并通过间接免疫荧光检测其亚细胞定位。在对照3T3成纤维细胞(生长对数后期)中,该酶仅位于细胞质中,而在H - ras转化细胞中,它大量暴露在细胞膜外侧。这一新发现强烈表明,致癌产物p2Iras能够诱导(或介导)PC - plc跨ras转化细胞的质膜转运,这不仅可能对细胞生物化学有影响(增强PC - plc活性,进而产生细胞内和细胞外的磷酸胆碱以及中性脂质积累),而且还可能对促进癌基因转化细胞的肿瘤侵袭和转移的细胞间相互作用机制有影响。
