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围产期奶牛肝脏中生长激素受体(GHR)信使核糖核酸减少是由GHR 1A的特异性下调引起的,这与胰岛素样生长因子I减少有关。

Reduced growth hormone receptor (GHR) messenger ribonucleic acid in liver of periparturient cattle is caused by a specific down-regulation of GHR 1A that is associated with decreased insulin-like growth factor I.

作者信息

Kobayashi Y, Boyd C K, Bracken C J, Lamberson W R, Keisler D H, Lucy M C

机构信息

Department of Animal Sciences, University of Missouri, Columbia 65211, USA.

出版信息

Endocrinology. 1999 Sep;140(9):3947-54. doi: 10.1210/endo.140.9.7000.

Abstract

GH receptor (GHR) messenger RNA (mRNA) is transcribed from at least three different promoters within the liver of cattle. The first promoter (P1) is liver specific and alternatively splices exon 1A onto the GHR mRNA (GHR 1A mRNA). The second and third promoters (P2 and P3) have constitutive activity in many tissues and alternatively splice exons 1B and 1C onto the GHR mRNA (GHR 1B and GHR 1C mRNA). The total amount of GHR in the liver partially determines liver insulin-like growth factor I (IGF-I) synthesis in response to GH. Two studies were conducted to characterize the changes in GHR 1A mRNA, alternatively spliced GHR mRNA, and IGF-I mRNA during late pregnancy and early lactation in dairy cattle. Liver RNA was isolated from pregnant Holstein cattle (Bos taurus) on days -14, 0, and 21 relative to parturition (study 1) or days -14, 0, 15, 30, 60, and 90 relative to parturition (study 2). Ribonuclease protection assays were used to quantify total GHR (all GHR variants) as well as liver-specific GHR 1A and alternatively spliced GHR mRNA. Likewise, total IGF-I as well as alternatively spliced IGF-I mRNA (class 1 and class 2 transcripts) were measured. A decrease in total GHR mRNA at parturition (P < 0.01) was associated with a specific decrease in GHR 1A mRNA (P < 0.001). The amount of alternatively spliced GHR mRNA (including GHR 1B and GHR 1C mRNA) did not change at parturition (P > 0.10). Total liver IGF-I mRNA and blood IGF-I concentrations were also decreased at parturition (P < 0.05 and P < 0.01, respectively). However, a decrease in IGF-I mRNA was observed for both class 1 and class 2 IGF-I transcripts (P < 0.01 and P < 0.05, respectively). We conclude that the reduced amount of GHR mRNA during early lactation is caused by a specific down-regulation of GHR 1A mRNA that was associated with decreased liver IGF-I mRNA and decreased blood IGF-I concentrations. These data provide evidence for independent regulation of GHR mRNA by mechanisms that discriminate between GHR P1 (transcribes GHR 1A) and alternative promoters that transcribe constitutive GHR mRNA.

摘要

生长激素受体(GHR)信使核糖核酸(mRNA)由牛肝脏内至少三种不同的启动子转录而来。第一个启动子(P1)具有肝脏特异性,可将外显子1A选择性剪接到GHR mRNA上(GHR 1A mRNA)。第二个和第三个启动子(P2和P3)在许多组织中具有组成型活性,并可将外显子1B和1C选择性剪接到GHR mRNA上(GHR 1B和GHR 1C mRNA)。肝脏中GHR的总量部分决定了肝脏中胰岛素样生长因子I(IGF-I)对生长激素的合成反应。进行了两项研究,以表征奶牛妊娠后期和泌乳早期GHR 1A mRNA、选择性剪接的GHR mRNA和IGF-I mRNA的变化。在相对于分娩的第-14、0和21天(研究1)或相对于分娩的第-14、0、15、30、60和90天(研究2),从怀孕的荷斯坦牛(Bos taurus)中分离肝脏RNA。采用核糖核酸酶保护试验来定量总GHR(所有GHR变体)以及肝脏特异性GHR 1A和选择性剪接的GHR mRNA。同样,测量了总IGF-I以及选择性剪接的IGF-I mRNA(1类和2类转录本)。分娩时总GHR mRNA的减少(P<0.01)与GHR 1A mRNA的特异性减少相关(P<0.001)。选择性剪接的GHR mRNA(包括GHR 1B和GHR 1C mRNA)的量在分娩时没有变化(P>0.10)。肝脏总IGF-I mRNA和血液IGF-I浓度在分娩时也降低(分别为P<0.05和P<0.01)。然而,1类和2类IGF-I转录本的IGF-I mRNA均减少(分别为P<0.01和P<0.05)。我们得出结论,泌乳早期GHR mRNA量的减少是由GHR 1A mRNA的特异性下调引起的,这与肝脏IGF-I mRNA减少和血液IGF-I浓度降低有关。这些数据为通过区分转录GHR 1A的GHR P1和转录组成型GHR mRNA 的替代启动子的机制对GHR mRNA进行独立调节提供了证据。

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