Montessuit C, Caverzasio J, Bonjour J P
Department of Medicine, University Hospital, Geneva, Switzerland.
J Biol Chem. 1991 Sep 25;266(27):17791-7.
The mechanisms by which calcium (Ca2+) and inorganic phosphate (Pi) accumulate into matrix vesicles (MV) have not been elucidated. In the present study the characteristics of Pi uptake into MV isolated from mildly rachitic chicken growth plate cartilage have been investigated. The results indicate that Pi accumulates into MV mainly via a Na(+)-dependent Pi transport system. In the absence of NaCl in the extravesicular medium, Pi uptake was a nonsaturable process. In the presence of 150 mM NaCl, the initial rate of Pi uptake was 4.38 +/- 1.02-fold higher than with 150 mM choline chloride (mean +/- S.E., n = 8, p less than 0.005). Other cations showed partial activity to drive Pi into MV as compared to Na+:Li+ (64.4%) greater than K+ (39.8%) greater than choline (39.0%) greater than tetramethylammonium (30.0%) greater than N-methylglucamine (26.3%). Na(+)-dependent Pi transport activity displayed saturability towards increasing extra-vesicular concentrations of Na+ and Pi. The apparent Km for Pi was 0.68 +/- 0.16 mM. The Na+ concentration producing half-maximum Pi transport activity was 106.2 +/- 11.0 mM. Kinetic analysis suggests that Na+ interacts with the Pi carrier with a stoichiometry of more than one Na+ ion with one Pi molecule. In MV isolated from normal chicken growth plate cartilage, this Na(+)-dependent Pi transport system was barely expressed. In contrast to the effect on Pi uptake by MV, the activity of alkaline phosphatase was not changed when NaCl was substituted for choline chloride in the assay medium. In addition to this observation which suggests that this enzyme is not related to the Pi transport activity described in this study, levamisole, which inhibited alkaline phosphatase activity did not affect the Na(+)-dependent uptake of Pi. Both arsenate and phosphonoformic acid, two inhibitors of the epithelial Na(+)-dependent Pi transport systems, were active inhibitors of the Na(+)-dependent Pi uptake by MV with a higher potency for phosphonoformic acid. Associated with the expression of a facilitated Na(+)-coupled Pi transport in MV, in vitro calcification assessed by 45Ca2+ uptake also showed a marked dependence on extravesicular sodium. This relationship was markedly attenuated in MV isolated from normal chicken growth plate cartilage expressing a weak Na(+)-facilitated Pi transport activity. In conclusion, a saturable Na(+)-dependent Pi carrier has been characterized which facilitates Pi transport in MV. Its potential role for Ca-Pi accumulation into MV and subsequent development of vesicular calcification followed by mineralization of the osteogenic matrix is proposed and remains to be further investigated.
钙(Ca2+)和无机磷酸盐(Pi)积聚到基质小泡(MV)中的机制尚未阐明。在本研究中,对从轻度佝偻病鸡生长板软骨中分离出的MV摄取Pi的特性进行了研究。结果表明,Pi主要通过依赖Na+的Pi转运系统积聚到MV中。在囊泡外介质中不存在NaCl时,Pi摄取是一个非饱和过程。在存在150 mM NaCl的情况下,Pi摄取的初始速率比存在150 mM氯化胆碱时高4.38±1.02倍(平均值±标准误,n = 8,p < 0.005)。与Na+相比,其他阳离子在驱动Pi进入MV方面表现出部分活性:Li+(64.4%)> K+(39.8%)> 胆碱(39.0%)> 四甲基铵(30.0%)> N-甲基葡糖胺(26.3%)。依赖Na+的Pi转运活性对囊泡外Na+和Pi浓度的增加表现出饱和性。Pi的表观Km为0.68±0.16 mM。产生半数最大Pi转运活性的Na+浓度为106.2±11.0 mM。动力学分析表明,Na+与Pi载体相互作用的化学计量为一个Pi分子对应不止一个Na+离子。在从正常鸡生长板软骨中分离出的MV中,这种依赖Na+的Pi转运系统几乎不表达。与对MV摄取Pi的影响相反,当在测定介质中用NaCl替代氯化胆碱时,碱性磷酸酶的活性没有改变。除了这一表明该酶与本研究中描述的Pi转运活性无关的观察结果外,抑制碱性磷酸酶活性的左旋咪唑不影响依赖Na+的Pi摄取。砷酸盐和膦甲酸这两种上皮细胞依赖Na+的Pi转运系统抑制剂,都是MV依赖Na+的Pi摄取的有效抑制剂,膦甲酸的效力更高。与MV中易化的Na+偶联Pi转运的表达相关,通过45Ca2+摄取评估的体外钙化也显示出对囊泡外钠的明显依赖性。在表达弱的Na+易化Pi转运活性的从正常鸡生长板软骨中分离出的MV中,这种关系明显减弱。总之,已鉴定出一种饱和的依赖Na+的Pi载体,它促进MV中的Pi转运。提出了其在Ca-Pi积聚到MV中以及随后囊泡钙化继而骨生成基质矿化中的潜在作用,有待进一步研究。
