内源性单adp核糖基化心脏蛋白通过抗adp核糖精氨酸免疫反应的证据。

C. J. Schwab, M. J. Colville, A. Fullerton, K. Mcmahon
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引用次数: 15

摘要

精氨酸特异性单adp核糖基化蛋白和精氨酸特异性单adp核糖基转移酶发生在心脏。我们开发了一种针对adp -核糖基聚精氨酸的多克隆抗血清R-28,该血清识别单adp -核糖基化蛋白,并鉴定了鹌鹑心脏的主要单adp -核糖基化产物。用羟胺处理固定蛋白结合的adp核糖基化的Gs蛋白,去除其精氨酸中的adp核糖,消除R-28对Gs的免疫反应性。此外,NaOH和磷酸二酯酶I处理可以去除R-28对鹌鹑心脏蛋白的免疫反应性。类似的氯化汞处理并没有消除免疫反应性,但确实从心脏Gi/Go蛋白的半胱氨酸中去除外源性(通过体外百日咳毒素处理)添加的adp核糖。抗血清与鹌鹑心脏制剂中的Rho的adp -核糖素天冬氨酸(由C3毒素形成)、延长因子2的adp -核糖素二苯二胺(由白喉毒素形成)或新生大鼠心脏制剂中的聚adp -核糖素蛋白没有反应。因此,R-28抗血清似乎主要含有针对adp -核糖精氨酸的抗体。为了验证R-28的有效性,我们对鹌鹑心脏亚细胞部分进行了免疫印迹。R-28在肌膜中表现出最大的免疫反应性,在较致密的膜组分中表现出显著的免疫反应性。胞质溶胶中还含有与细胞膜中发现的不同的免疫反应带。羟胺处理消除了肌膜和致密膜部分的免疫反应性,但没有消除细胞质,表明膜免疫反应带含有adp -核糖精氨酸。总之,建立了一种识别adp -核糖精氨酸蛋白的多克隆抗血清。鹌鹑心脏内源性精氨酸单adp核糖基化产物的表征证明了抗血清的有效性。鹌鹑心脏有几个肌层和致密的膜部分蛋白,似乎是单adp核糖基化在精氨酸上。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Evidence of endogenous mono-ADP-ribosylation of cardiac proteins via anti-ADP-ribosylarginine immunoreactivity.
Arginine-specific mono-ADP-ribosylation of proteins and arginine-specific mono-ADP-ribosyltransferase occur in heart. We developed a polyclonal antiserum, R-28, against ADP-ribosylpolyarginine that recognized mono-ADP-ribosylated proteins and identified the major mono-ADP-ribosylation products of quail heart. Treatment of Immobilon-bound ADP-ribosylated Gs protein with hydroxylamine under conditions that remove ADP-ribose from its arginines eliminated R-28 immunoreactivity to Gs. Also, R-28 immunoreactivity to quail heart proteins was removed by NaOH and phosphodiesterase I treatments. Similar treatment with mercuric chloride did not remove the immunoreactivity but did remove exogenously (via in vitro pertussis toxin treatment) added ADP-ribose from cysteine of cardiac Gi/Go proteins. The antiserum did not appear to react with ADP-ribosylasparagine of Rho (formed by C3 toxin), ADP-ribosyldiphthamide of elongation factor 2 (formed by diphtheria toxin) in quail heart preparations, or polyADP-ribosylated proteins of a neonate rat cardiac nuclear preparation. Thus, the R-28 antiserum appears to contain predominantly antibodies directed against ADP-ribosylarginine. To test the usefulness of R-28, immunoblotting of subcellular fractions of quail heart was performed. R-28 showed the greatest immunoreactivity in the sarcolemma with significant immunoreactivity in denser membrane fractions. The cytosol also contained an immunoreactive band distinct from those found in the membranes. Hydroxylamine treatment eliminated immunoreactivity in the sarcolemma and denser membrane fractions but not the cytosol, suggesting the membranous immunoreactive bands contain ADP-ribosylarginine. In conclusion, a polyclonal antiserum that recognizes ADP-ribosylarginine proteins has been raised. The usefulness of the antiserum is demonstrated by the characterization of endogenous arginine mono-ADP-ribosylation products in quail heart. The quail heart has several sarcolemmal and denser membrane fraction proteins that appear to be mono-ADP-ribosylated on arginines.
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