Garcia-Sancho J, Sanchez A, Christensen H N
Biochim Biophys Acta. 1977 Jan 21;464(2):295-312. doi: 10.1016/0005-2736(77)90005-0.
The pH profile for the uptake of L-glutamic acid by the Ehrlich ascites tumor cell arises largely as a sum of the decline with falling pH of a slow, Na+-dependent uptake by System A, and an increasing uptake by Na+-independent System L. The latter maximizes at about pH 4.5, following approximately the titration curve of the distal carboxyl group. This shift in route of uptake was verified by (a) a declining Na+-dependent component, (b) an almost corresponding decline in the 2-(methylamino)-isobutyric acid-inhibitable component, (c) a rising component inhibited by 2-aminonorbornane-2-carboxylic acid. Other amino acids recognized as principally reactive with Systems A or L yielded corresponding inhibitory effects with some conspicious exceptions: 2-Aminoisobutyric acid and even glycine become better substrates of System L as the pH is lowered; hence their inhibitory action on glutamic acid uptake is not lost. The above results were characterized by generally consistent relations among the half-saturation concentrations of the interacting amino acids with respect to: their own uptake, their inhibition of the uptake, one by another, and their trans stimulation of exodus, one by another. A small Na+-dependent component of uptake retained by L-glutamic acid but not by D-glutamic acid at pH 4.5 is inhibitable by methionine but by neither 2-(methylamino)-isobutyric acid nor the norbornane amino acid. We provisionally identified this component with System ASC, which transports L-glutamine throughout the pH range studied. No transport activity specific to the anionic amino acids was detected, and the unequivocally anionic cysteic acid showed neither significant mediated uptake nor inhibition of the uptake of glutamic aic or of the norbornane amino acid. The dicarboxylic amino acids take the sequence, aspartic acid less than glutamic acid less than alpha-aminoadipic acid less than S-carboxymethylcysteine, in their rate of mediated, Na+-independent uptake at low pH. Diiodotyrosine and two dissimilas isomers of nitrotyrosine also show acceleration of uptake as the phenolate group on the sidechain is protonated, a result indicating that the acidic group need not be a carboxyl group and need not take a specific position in space to be accepted at the receptor site L. The presence of the carboxyl group does not upset the normal stereospecificity of System L until it falls on the beta-carbon in aspartic acid; even then it is the presence of the carbonyl group and not of the intact carboxyl group nor of its hydroxyl group that cancels out the stereospecificity, as was shown by the absence of normal stereospecificity for aspartic acid and asparagine and its presence in glutamic acid, homoserine and glutamine. In agreement, the uptak of aspartic acid is peculiarly sensitive to the presence of an alpha-methyl group or of other structures that modify the orientation of the sidechain.
艾氏腹水瘤细胞摄取L-谷氨酸的pH曲线,很大程度上是由以下两部分组成:随着pH值下降,系统A介导的缓慢的、依赖Na⁺的摄取下降;以及不依赖Na⁺的系统L介导的摄取增加。后者在约pH 4.5时达到最大值,大致遵循远端羧基的滴定曲线。摄取途径的这种转变通过以下几点得到证实:(a) 依赖Na⁺的成分下降;(b) 2-(甲氨基)-异丁酸可抑制的成分几乎相应下降;(c) 被2-氨基降冰片烷-2-羧酸抑制的成分上升。其他主要被认为与系统A或L有反应的氨基酸也产生了相应抑制作用,但有一些明显的例外:随着pH值降低,2-氨基异丁酸甚至甘氨酸成为系统L更好的底物;因此它们对谷氨酸摄取的抑制作用并未丧失。上述结果的特点是,相互作用的氨基酸在以下方面的半数饱和浓度之间存在普遍一致的关系:它们自身的摄取、它们对彼此摄取的抑制以及它们对彼此外流的转刺激。在pH 4.5时,L-谷氨酸保留了一小部分依赖Na⁺的摄取成分,而D-谷氨酸则没有,该成分可被甲硫氨酸抑制,但不能被2-(甲氨基)-异丁酸或降冰片烷氨基酸抑制。我们暂时将该成分确定为系统ASC,它在整个研究的pH范围内转运L-谷氨酰胺。未检测到对阴离子氨基酸有特异性的转运活性,明确为阴离子的半胱氨酸对谷氨酸或降冰片烷氨基酸的摄取既无显著的介导摄取作用,也无抑制作用。在低pH下,二羧酸氨基酸介导的、不依赖Na⁺的摄取速率顺序为:天冬氨酸<谷氨酸<α-氨基己二酸<S-羧甲基半胱氨酸。二碘酪氨酸和两种硝基酪氨酸的不同异构体也显示,随着侧链上酚羟基质子化,摄取加速,这一结果表明酸性基团不一定是羧基,也不一定在空间中占据特定位置就能被受体位点L接受。羧基的存在不会破坏系统L正常的立体特异性,除非它位于天冬氨酸的β-碳上;即便如此,正如天冬氨酸和天冬酰胺缺乏正常立体特异性而谷氨酸、高丝氨酸和谷氨酰胺具有正常立体特异性所表明的那样,是羰基的存在而非完整羧基或其羟基的存在消除了立体特异性。与此一致的是,天冬氨酸的摄取对α-甲基或其他改变侧链取向的结构的存在特别敏感。
Zotero 插件