U-73122是一种氨基甾体磷脂酶C拮抗剂,它能非竞争性抑制生长激素释放激素对GH3大鼠垂体细胞的作用。
U-73122, an aminosteroid phospholipase C antagonist, noncompetitively inhibits thyrotropin-releasing hormone effects in GH3 rat pituitary cells.
作者信息
Smallridge R C, Kiang J G, Gist I D, Fein H G, Galloway R J
机构信息
Department of Clinical Physiology, Walter Reed Army Institute of Research, Washington, D.C. 20307-5100.
出版信息
Endocrinology. 1992 Oct;131(4):1883-8. doi: 10.1210/endo.131.4.1396332.
TRH increases cytosolic-free calcium ([Ca2+]i) by activating phospholipase C(PL-C), which induces phosphoinositol hydrolysis, leading to Ca2+ mobilization from inositol trisphosphate (IP3) sensitive stores, and by increasing Ca2+ influx. Increases in [Ca2+]i stimulate PRL secretion. We investigated the effects of U-73122, an aminosteroid inhibitor of PL-C dependent processes, on TRH-stimulated second messenger pathways and on PRL secretion in GH3 rat pituitary cells. [Ca2+]i was monitored by Indo-1 fluorescence, and IP3 and metabolites separated on ion exchange columns. In Ca(2+)-free buffer, [Ca2+]i was 96 +/- 6 nM and increased to 323 +/- 23 nM (P less than 0.001) after TRH (100 nM). U-73122 dose dependently inhibited the TRH effect (IC50 = 967 nM; complete inhibition at 3-5 microM). Subsequent addition of monensin (100 microM) increased [Ca2+]i from 107 +/- 4 to 142 +/- 4 nM (P < 0.001), confirming our previous findings of a non-TRH regulated Ca2+ pool in GH3 cells. Pretreatment (15 sec) with U-73122 partly inhibited the TRH effect on [Ca2+]i; complete suppression occurred with 70 sec of pretreatment. An inactive analog (U-73343) had no inhibitory effect at 5 microM. U-73122 acted noncompetitively, as the mean maximum velocity (expressed as percent increase in [Ca2+]i after TRH) was reduced from 225 to 91 while the Michaelis-Menten constant for TRH was unchanged (15.4 vs. 13.8 nM, n = 3). Of note, U-73122, at 3-5 microM, increased basal [Ca2+]i from 109 +/- 5 to 120 +/- 5 nM (P less than 0.001). In 1.3 mM Ca2+ buffer containing nifedipine (1 microM) and verapamil (50 microM), similar effects of U-73122 (5 microM) were observed on basal and TRH-stimulated [Ca2+]i. IP3, IP2, and IP1 increased to 241 +/- 12%, 148 +/- 23%, and 167 +/- 39% of control, 30 sec after TRH (100 nM); these responses were prevented by 1 microM U-73122. At 5 microM, U-73122 also significantly increased IP3 levels. TRH (100 nM) increased 4-h PRL secretion from 16.3 +/- 1.4 to 27.6 +/- 3.2 ng/well (P less than 0.05). U-73122 (5 microM) increased basal PRL secretion to 35.9 +/- 3.2 ng/well (P less than 0.05), but abolished the TRH effect. In contrast, U-73343 (with Ca2+ channel blockers) did not inhibit the TRH effect on PRL (control: 24.3 +/- 2.1; TRH: 51.0 +/- 6.3 ng/well).(ABSTRACT TRUNCATED AT 400 WORDS)
促甲状腺激素释放激素(TRH)通过激活磷脂酶C(PL - C)增加胞质游离钙([Ca2+]i),这会诱导磷酸肌醇水解,导致Ca2+从三磷酸肌醇(IP3)敏感储存库中释放,并增加Ca2+内流。[Ca2+]i的增加刺激催乳素(PRL)分泌。我们研究了U - 73122(一种PL - C依赖性过程的氨基类固醇抑制剂)对TRH刺激的第二信使途径以及对GH3大鼠垂体细胞中PRL分泌的影响。通过Indo - 1荧光监测[Ca2+]i,并在离子交换柱上分离IP3及其代谢产物。在无钙缓冲液中,[Ca2+]i为96±6 nM,TRH(100 nM)作用后增加至323±23 nM(P<0.001)。U - 73122剂量依赖性地抑制TRH的作用(IC50 = 967 nM;3 - 5μM时完全抑制)。随后加入莫能菌素(100μM)使[Ca2+]i从107±4 nM增加至142±4 nM(P<0.001),证实了我们之前关于GH3细胞中存在非TRH调节的Ca2+池的发现。用U - 73122预处理(15秒)部分抑制了TRH对[Ca2+]i的作用;预处理70秒时完全抑制。无活性类似物(U - 73343)在5μM时无抑制作用。U - 73122起非竞争性作用,因为平均最大速度(表示为TRH作用后[Ca2+]i的增加百分比)从225降至91,而TRH的米氏常数未改变(分别为15.4和13.8 nM,n = 3)。值得注意的是,3 - 5μM的U - 73122使基础[Ca2+]i从109±5 nM增加至120±5 nM(P<0.001)。在含有硝苯地平(1μM)和维拉帕米(50μM)的1.3 mM钙缓冲液中,观察到U - 73122(5μM)对基础和TRH刺激的[Ca2+]i有类似作用。TRH(100 nM)作用30秒后,IP3、IP2和IP1分别增加至对照的241±12%、148±23%和167±39%;这些反应被1μM的U - 73122阻断。在5μM时,U - 73122也显著增加IP3水平。TRH(100 nM)使4小时PRL分泌从16.3±1.4 ng/孔增加至27.6±3.2 ng/孔(P<0.05)。U - 73122(5μM)使基础PRL分泌增加至35.9±3.2 ng/孔(P<0.05),但消除了TRH的作用。相比之下,U - 73343(与钙通道阻滞剂一起)不抑制TRH对PRL的作用(对照:24.3±2.1;TRH:51.0±6.3 ng/孔)。(摘要截断于400字)
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