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兔泪腺腺泡的分离及亚细胞分级分离分析

Isolation and subcellular fractionation analysis of acini from rabbit lacrimal glands.

作者信息

Bradley M E, Lambert R W, Lambert R W, Lee L M, Mircheff A K

机构信息

Department of Physiology and Biophysics, University of Southern California School of Medicine, Los Angeles 90033.

出版信息

Invest Ophthalmol Vis Sci. 1992 Sep;33(10):2951-65.

PMID:1326495
Abstract

The rabbit has been a useful model for in vivo studies of the pharmacologic control of lacrimal gland fluid secretion. However, by contrast with rodent exorbital lacrimal glands, the rabbit lacrimal gland has not been subjected to detailed cellular, subcellular, or biochemical analyses. Procedures were developed to isolate rabbit lacrimal acini by collagenase digestion and mechanical dispersion. The preparations exhibited good morphology, and trypan blue exclusion rates generally exceeded 90%. The isolated acini responded to carbachol by releasing protein and increasing Na+ unidirectional influx rates. The presence of muscarinic cholinergic and beta-adrenergic receptors was indicated by specific binding of the muscarinic cholinergic antagonist, 3H-N-methylscopolamine (3H-NMS; dissociation constant, Kd, 0.55 nmol/l), and the beta-adrenergic antagonist, 3H-CGP12177 (Kd, 0.34 nmol/l). The maximal binding values measured in crude membrane preparations were 79 fmol/mg for 3H-NMS and 40 fmol/mg for 3H-CGP12177. Subcellular fractionation analyses showed various membrane populations, including a series of Golgi-derived populations admixed with a major endoplasmic reticulum-derived population, a population that may represent the basal-lateral plasma membranes, and a series of populations with characteristics suggesting they are involved in the assembly or recycling of basal-lateral membrane constituents. The authors believe the ability to isolate and analyze acinar preparations from the rabbit lacrimal gland will facilitate various studies of acinar cell biochemistry and physiology that would be impractical with the relatively smaller amounts of material that can be obtained from rat or mouse exorbital lacrimal glands.

摘要

兔子一直是泪腺液分泌药理控制体内研究的有用模型。然而,与啮齿动物的眶外泪腺不同,兔子泪腺尚未进行详细的细胞、亚细胞或生化分析。已开发出通过胶原酶消化和机械分散来分离兔泪腺腺泡的方法。制备物显示出良好的形态,台盼蓝排斥率通常超过90%。分离出的腺泡对卡巴胆碱有反应,表现为释放蛋白质和增加钠的单向流入速率。毒蕈碱胆碱能拮抗剂3H-N-甲基东莨菪碱(3H-NMS;解离常数Kd为0.55 nmol/l)和β-肾上腺素能拮抗剂3H-CGP12177(Kd为0.34 nmol/l)的特异性结合表明存在毒蕈碱胆碱能和β-肾上腺素能受体。在粗膜制剂中测得的最大结合值,3H-NMS为79 fmol/mg,3H-CGP12177为40 fmol/mg。亚细胞分级分离分析显示了各种膜群体,包括一系列与主要内质网衍生群体混合的高尔基体衍生群体、一个可能代表基底外侧质膜的群体,以及一系列具有表明它们参与基底外侧膜成分组装或再循环特征的群体。作者认为,从兔泪腺分离和分析腺泡制剂的能力将促进对腺泡细胞生物化学和生理学的各种研究,而从大鼠或小鼠眶外泪腺获得的材料相对较少,进行这些研究将不切实际。

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