Steinberg T H, Newman A S, Swanson J A, Silverstein S C
J Biol Chem. 1987 Jun 25;262(18):8884-8.
Extracellular ATP induces cation fluxes in thioglycolate-elicited mouse peritoneal macrophages and the J774 macrophage cell line apparently due to ligation of a plasma membrane receptor for ATP4-. We report that ATP permeabilizes the plasma membrane of J774 cells to 6-carboxyfluorescein (376 Da), lucifer yellow (457 Da), and fura-2 (831 Da) but not to trypan blue (961 Da), Evans blue (961 Da), or larger dye conjugates. We employed fluorescence microscopy and quantitative fluorimetry to study entry of lucifer yellow into the cytoplasm of J774 cells. Permeabilization to lucifer yellow appears to be mediated by the same ATP4- receptor that induces cation fluxes because it was inhibited by divalent cations and low pH, was mediated by the nonhydrolyzable analog adenosine 5'-(beta, gamma-imido)triphosphate, and because a variant J774 cell line resistant to ATP-induced Rb+ efflux did not take up lucifer yellow when exposed to ATP. ATP permeabilization was reversed within 5 min by removal of ATP or by addition of divalent cations. ATP also caused a transient increase in lucifer yellow uptake by pinocytosis. These data suggest that ATP4- ligates a receptor on macrophages which induces the formation of a channel admitting molecules less than or equal to 831 daltons into the cytoplasmic matrix and that removal of ATP4- from the medium causes rapid channel closure.
细胞外ATP可诱导经巯基乙酸盐激发的小鼠腹腔巨噬细胞和J774巨噬细胞系出现阳离子通量,这显然是由于ATP4-的质膜受体的结合所致。我们报道,ATP可使J774细胞的质膜对6-羧基荧光素(376道尔顿)、路西法黄(457道尔顿)和fura-2(831道尔顿)通透,但对台盼蓝(961道尔顿)、伊文思蓝(961道尔顿)或更大的染料偶联物不通透。我们采用荧光显微镜和定量荧光测定法来研究路西法黄进入J774细胞胞质的情况。对路西法黄的通透似乎是由诱导阳离子通量的同一ATP4-受体介导的,因为它受到二价阳离子和低pH的抑制,由不可水解的类似物腺苷5'-(β,γ-亚氨基)三磷酸介导,并且因为对ATP诱导的Rb+外流有抗性的J774细胞系变体在暴露于ATP时不摄取路西法黄。通过去除ATP或添加二价阳离子,ATP通透作用在5分钟内逆转。ATP还通过胞饮作用导致路西法黄摄取短暂增加。这些数据表明,ATP4-与巨噬细胞上的一种受体结合,该受体诱导形成一个通道,允许小于或等于831道尔顿的分子进入细胞质基质,并且从培养基中去除ATP4-会导致通道迅速关闭。
