Wichelhaus D P, Jones C T
Laboratory of Cellular and Developmental Physiology, University of Oxford, John Radcliffe Hospital, UK.
J Dev Physiol. 1992 Aug;18(2):49-58.
The nature distribution and associated GTP gamma S binding activity of phosphatidylinositol phospholipase C (PI-PLC) has been studied in non-pregnant and pregnant guinea pig uterine smooth muscle. Cytosolic fractions partially purified by Q-Sepharose and heparin-Agarose chromatography show two isoenzyme forms, one with an apparent molecular weight of 58 kD that crossreacts with PI-PLC alpha and a has Km for phosphatidylinositol of 292 +/- 72.6 microM, designated alpha, and a form that has an apparent molecular weight of 86 kD and a substrate Km of 54 +/- 20 microM designated delta. Approximately 80% of the total PI-PLC activity was recovered in the cytosolic fraction and this increased 8-10 fold for both isoenzymes from the non-pregnant to the late pregnant uterus and the proportion of the alpha isoenzyme increased from approximately 40% to 55% of the total. PI-PLC alpha but not delta activity had GTP gamma S binding activity associated with it after Q-Sepharose or heparin-Agarose chromatography. This associated activity accounted for 2% of the total GTP gamma S-binding activity in the non-pregnant uterus and 31% of that in the near-term uterus. On separation of the PI-PLCa-GTP gamma S-binding complex by gel filtration on Sephacryl S200 gave two peaks one of 118 kD accounting for two-thirds of all the binding and two-thirds of the enzyme activity and a 58 kD peak. The 118 kD peak could not be separated by treatment with 0.5% cholate, but in this form enzyme activity was protected from detergent inactivation found with the 58 kD form. In sodium dodecyl sulphate polyacrylamide-gel electrophoresis PI-PLC alpha was released from the 118 kD complex and showed an apparent molecular weight of 61.5 kD. All the activity in the residual membrane fraction could be released by washing with buffer followed by, 2 M KCl and then 2 M KCl plus 0.5% cholate. This released isoenzyme forms that appeared identical to those in the cytosolic fraction and with GTP gamma S-binding activity associated with PI-PLC alpha. It is concluded that in the near term guinea pig uterus there is a dramatic increase in the capacity for inositol polyphosphate production. Moreover the dramatic increase in GTP gamma S-binding activity associated with PI-PLC alpha implies large changes in the extent and possibly nature of the putative G-protein activation of this pathway.(ABSTRACT TRUNCATED AT 400 WORDS)
在未孕和孕豚鼠子宫平滑肌中,对磷脂酰肌醇磷脂酶C(PI-PLC)的性质分布及相关的GTPγS结合活性进行了研究。通过Q-琼脂糖凝胶和肝素-琼脂糖凝胶色谱法部分纯化的胞质组分显示出两种同工酶形式,一种表观分子量为58kD,与PI-PLCα发生交叉反应,对磷脂酰肌醇的Km为292±72.6μM,称为α型;另一种表观分子量为86kD,底物Km为54±20μM,称为δ型。约80%的总PI-PLC活性存在于胞质组分中,从未孕子宫到妊娠晚期子宫,两种同工酶的活性均增加了8-10倍,α同工酶在总量中的比例从约40%增加到55%。在Q-琼脂糖凝胶或肝素-琼脂糖凝胶色谱后,PI-PLCα活性而非δ活性具有与之相关的GTPγS结合活性。这种相关活性在未孕子宫中占总GTPγS结合活性的2%,在足月子宫中占31%。通过Sephacryl S200凝胶过滤分离PI-PLCα-GTPγS结合复合物时出现两个峰,一个118kD的峰占所有结合的三分之二和酶活性的三分之二,另一个58kD的峰。用0.5%胆酸盐处理无法分离118kD的峰,但这种形式的酶活性可免受58kD形式所发现的去污剂失活影响。在十二烷基硫酸钠聚丙烯酰胺凝胶电泳中,PI-PLCα从118kD复合物中释放出来,表观分子量为61.5kD。残留膜组分中的所有活性可通过用缓冲液洗涤,然后用2M KCl洗涤,再用2M KCl加0.5%胆酸盐洗涤而释放。释放出的同工酶形式与胞质组分中的相同,并具有与PI-PLCα相关的GTPγS结合活性。结论是,在妊娠晚期豚鼠子宫中,肌醇多磷酸生成能力显著增加。此外,与PI-PLCα相关的GTPγS结合活性的显著增加意味着该途径假定的G蛋白激活程度及可能的性质发生了巨大变化。(摘要截短至400字)
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