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羟胺对视杆光感受器中抑制蛋白(S抗原)亚细胞分布的影响。

Effect of hydroxylamine on the subcellular distribution of arrestin (S-antigen) in rod photoreceptors.

作者信息

Mangini N J, Garner G L, Okajima T I, Donoso L A, Pepperberg D R

机构信息

Department of Ophthalmology and Visual Sciences, Lions of Illinois Eye Research Institute, University of Illinois, Chicago College of Medicine.

出版信息

Vis Neurosci. 1994 May-Jun;11(3):561-8. doi: 10.1017/s0952523800002467.

Abstract

The immunocytochemical labeling of arrestin (S-antigen) in photoreceptors of the ovine retina was examined following incubation of the retina with hydroxylamine (NH2OH), an agent known to inhibit the phosphorylation of photoactivated rhodopsin. Intact, isolated retinas bathed in medium containing 20 mM NH2OH, or in control medium lacking NH2OH, were maintained in darkness or exposed to bright light for 3 min (dark-adapted and light-adapted conditions, respectively); further incubated in darkness for 10 min; and then fixed and prepared for cryosectioning. Cryosections were incubated with anti-S-antigen monoclonal antibody MAb A2G5; with secondary antibodies that were conjugated with horseradish peroxidase; and with either 3-amino-9-ethyl carbazole or diaminobenzidine as chromogen. Anti-arrestin labeling in cryosections was then analyzed densitometrically using a light-microscopic image processing system. In dark-adapted control retinas, labeling density of the photoreceptor outer segment (OS) layer (0.061 +/- 0.004; average +/- S.E.M.) was less than that of the inner segment (IS) layer (0.138 +/- 0.011). In light-adapted control retinas, OS labeling density (0.139 +/- 0.007) exceeded IS labeling density (0.095 +/- 0.005). Incubation with NH2OH eliminated this light-dependent increase in labeling of the OS relative to that of the IS, i.e. eliminated the increase in relative OS/IS labeling. Densities of labeling were 0.110 +/- 0.006 (OS) and 0.183 +/- 0.006 (IS) in NH2OH-treated dark-adapted retinas vs. 0.078 +/- 0.004 (OS) and 0.182 +/- 0.008 (IS) in NH2OH-treated light-adapted retinas. Anti-arrestin labeling was also examined in retinas that were exposed to 3 min or 13 min of bright light and then immediately fixed.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在用已知可抑制光活化视紫红质磷酸化的试剂羟胺(NH₂OH)孵育绵羊视网膜后,检测了视锥蛋白(S - 抗原)在绵羊视网膜光感受器中的免疫细胞化学标记。将完整的离体视网膜置于含有20 mM NH₂OH的培养基中,或置于不含NH₂OH的对照培养基中,分别在黑暗中或暴露于强光下3分钟(分别为暗适应和光适应条件);再在黑暗中孵育10分钟;然后固定并制备用于冷冻切片。冷冻切片与抗S - 抗原单克隆抗体MAb A2G5孵育;与与辣根过氧化物酶偶联的二抗孵育;并用3 - 氨基 - 9 - 乙基咔唑或二氨基联苯胺作为显色剂。然后使用光学显微镜图像处理系统对冷冻切片中的抗视锥蛋白标记进行光密度分析。在暗适应的对照视网膜中,光感受器外段(OS)层的标记密度(0.061±0.004;平均值±标准误)低于内段(IS)层(0.138±0.011)。在光适应的对照视网膜中,OS标记密度(0.139±0.007)超过IS标记密度(0.095±0.005)。用NH₂OH孵育消除了相对于IS而言OS标记的这种光依赖性增加,即消除了相对OS/IS标记的增加。在经NH₂OH处理的暗适应视网膜中,标记密度为0.110±0.006(OS)和0.183±0.006(IS),而在经NH₂OH处理的光适应视网膜中为0.078±0.004(OS)和0.182±0.008(IS)。还在暴露于3分钟或13分钟强光然后立即固定的视网膜中检测了抗视锥蛋白标记。(摘要截断于250字)

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