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对照受试者和乳糜泻患者空肠活检组织体外培养过程中亚细胞器的碱性磷酸酶合成及特性

Alkaline phosphatase synthesis and properties of subcellular organelles during in vitro culture of jejunal biopsies from control subjects and patients with coeliac disease.

作者信息

Jones P E, L'Hirondel C, Peters T J

出版信息

Gut. 1982 Feb;23(2):108-14. doi: 10.1136/gut.23.2.108.

Abstract

Portions of jejunal biopsies from control subjects and from patients with coeliac disease were cultured for 24 hours using an in vitro organ culture technique. Alkaline phosphatase activity was measured in the tissue and medium before and after culture; enzyme activities were expressed per microgram tissue DNA. The increase in enzyme activity during the culture period was taken to represent net enzyme synthesis. Alkaline phosphatase synthesis by mucosa from patients with untreated gluten-sensitive coeliac disease and by mucosa from patients with non-responsive coeliac disease was significantly less than that by normal mucosa. Alkaline phosphatase synthesis by mucosa from patients with treated gluten-sensitive coeliac disease was greater than that by untreated coeliac mucosa but was less than normal mucosa. Sequential studies of alkaline phosphatase synthesis by jejunal mucosa from seven patients with coeliac disease, before and after successful treatment by gluten withdrawal, showed an increase in synthesis in all patients. Study, by analytical subcellular fractionation with sucrose density gradient centrifugation, of the properties of the organelles of cultured control tissue showed good preservation of their integrity. A striking finding, however, was the decrease in malate dehydrogenase with a corresponding marked increase in lactate dehydrogenase. This would be expected to be followed by a shift from aerobic to anaerobic metabolism. Analytical subcellular fractionation of cultured mucosa from patients with coeliac disease gave similar conclusions. There was, however, a marked improvement of the brush border abnormalities, characteristic of coeliac disease, during culture with increased enzyme activities and membrane equilibrium density in the sucrose gradients.

摘要

采用体外器官培养技术,将来自对照受试者和乳糜泻患者的部分空肠活检组织培养24小时。在培养前后分别测定组织和培养基中的碱性磷酸酶活性;酶活性以每微克组织DNA表示。培养期间酶活性的增加被视为净酶合成。未经治疗的麸质敏感型乳糜泻患者的黏膜和无反应性乳糜泻患者的黏膜合成碱性磷酸酶的能力明显低于正常黏膜。经治疗的麸质敏感型乳糜泻患者的黏膜合成碱性磷酸酶的能力高于未经治疗的乳糜泻黏膜,但低于正常黏膜。对7例乳糜泻患者在成功戒食麸质治疗前后空肠黏膜合成碱性磷酸酶的情况进行的系列研究表明,所有患者的合成能力均有所增加。通过蔗糖密度梯度离心进行分析性亚细胞分级分离,对培养的对照组织细胞器的特性进行研究,结果显示其完整性得到了良好的保存。然而,一个显著的发现是苹果酸脱氢酶减少,同时乳酸脱氢酶相应显著增加。预计这将伴随着从有氧代谢向无氧代谢的转变。对乳糜泻患者培养的黏膜进行分析性亚细胞分级分离得出了类似的结论。然而,在培养过程中,乳糜泻特有的刷状缘异常有了显著改善,同时酶活性增加,蔗糖梯度中的膜平衡密度也增加。

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