豚鼠突触体中钙激活的磷脂酰肌醇4-磷酸和磷脂酰肌醇4,5-二磷酸的水解作用

Calcium-activated hydrolysis of phosphatidyl-myo-inositol 4-phosphate and phosphatidyl-myo-inositol 4,5-bisphosphate in guinea-pig synaptosomes.

作者信息

Griffin H D, Hawthorne J N

出版信息

Biochem J. 1978 Nov 15;176(2):541-52. doi: 10.1042/bj1760541.

DOI:10.1042/bj1760541

PMID:217364

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1186263/

Abstract

Addition of the bivalent ionophore A23187 to synaptosomes isolated from guinea-pig brain cortex and labelled with [(32)P]phosphate in vitro or in vivo caused a marked loss of radioactivity from phosphatidyl-myo-inositol 4-phosphate (diphosphoinositide) and phosphatidyl-myo-inositol 4,5-bisphosphate (triphosphoinositide) and stimulated labelling of phosphatidate. No change occurred in the labelling of other phospholipids. 2. In conditions that minimized changes in internal Mg(2+) concentrations, the effect of ionophore A23187 on labelling of synaptosomal di- and tri-phosphoinositide was dependent on Ca(2+) and was apparent at Ca(2+) concentrations in the medium as low as 10(-5)m. 3. An increase in internal Mg(2+) concentration stimulated incorporation of [(32)P]phosphate into di- and tri-phosphoinositide, whereas lowering internal Mg(2+) decreased labelling. 4. Increased labelling of phosphatidate was independent of medium Mg(2+) concentration and apparently only partly dependent on medium Ca(2+) concentration. 5. The loss of label from di- and tri-phosphoinositide caused by ionophore A23187 was accompanied by losses in the amounts of both lipids. 6. Addition of excess of EGTA to synaptosomes treated with ionophore A23187 in the presence of Ca(2+) caused a rapid resynthesis of di- and tri-phosphoinositide and a further stimulation of phosphatidate labelling. 7. Addition of ionophore A23187 to synaptosomes labelled in vivo with [(3)H]inositol caused a significant loss of label from di- and tri-phosphoinositide, but not from phosphatidylinositol. There was a considerable rise in labelling of inositol diphosphate, a small increase in that of inositol phosphate, but no significant production of inositol triphosphate. 8. (32)P-labelled di- and tri-phosphoinositides appeared to be located in the synaptosomal plasma membrane. 9. The results indicate that increased Ca(2+) influx into synaptosomes markedly activates triphosphoinositide phosphatase and diphosphoinositide phosphodiesterase, but has little or no effect on phosphatidylinositol phosphodiesterase.

摘要

向从豚鼠脑皮层分离并在体外或体内用[³²P]磷酸盐标记的突触体中添加二价离子载体A23187，导致磷脂酰肌醇4 - 磷酸（二磷酸肌醇）和磷脂酰肌醇4,5 - 二磷酸（三磷酸肌醇）的放射性显著丧失，并刺激了磷脂酸的标记。其他磷脂的标记没有变化。2. 在使内部镁离子浓度变化最小化的条件下，离子载体A23187对突触体二磷酸和三磷酸肌醇标记的影响取决于钙离子，并且在培养基中钙离子浓度低至10⁻⁵m时就很明显。3. 内部镁离子浓度的增加刺激了[³²P]磷酸盐掺入二磷酸和三磷酸肌醇，而降低内部镁离子浓度则减少了标记。4. 磷脂酸标记的增加与培养基镁离子浓度无关，显然仅部分依赖于培养基钙离子浓度。5. 离子载体A23187导致的二磷酸和三磷酸肌醇标记的丧失伴随着这两种脂质含量的减少。6. 在钙离子存在下，向用离子载体A23187处理的突触体中添加过量的乙二醇双四乙酸（EGTA），导致二磷酸和三磷酸肌醇迅速重新合成，并进一步刺激磷脂酸标记。7. 向在体内用[³H]肌醇标记的突触体中添加离子载体A23187，导致二磷酸和三磷酸肌醇的标记显著丧失，但磷脂酰肌醇没有。肌醇二磷酸的标记有相当大的增加，肌醇磷酸的标记有小幅增加，但肌醇三磷酸没有显著产生。8. ³²P标记的二磷酸和三磷酸肌醇似乎位于突触体的质膜中。9. 结果表明，突触体中钙离子内流增加显著激活了三磷酸肌醇磷酸酶和二磷酸肌醇磷酸二酯酶，但对磷脂酰肌醇磷酸二酯酶几乎没有影响。