Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture
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Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture
Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture
解放军医学杂志(英文版)2002年第3期 页码:167-170
Affiliations:
1. Department of Radiology
2. Xijing Hospital
3. Tangdu Hospital
4. Department of Stomatology Biology
5. Qindu Stomatology Hospital
6. Department of anatomy
7. Department of Biochemistry
8. Fourth Military Medical University
9. ,China
Author bio:
Funds:
DOI:
中图分类号:R33
纸质出版:2002
Accepted:
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Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture[J]. 解放军医学杂志(英文版), 2002,(3):167-170.
[1]张劲松,魏经国,吴军正,张淼丽,王丹,纪宗玲.Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture[J].Journal of Medical Colleges of PLA,2002(03):167-170+209.
Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture[J]. 解放军医学杂志(英文版), 2002,(3):167-170.DOI:
[1]张劲松,魏经国,吴军正,张淼丽,王丹,纪宗玲.Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture[J].Journal of Medical Colleges of PLA,2002(03):167-170+209.DOI:
Effects of cholesterol liposomes on cytoskeleton and proliferation of rabbit sphincter of Oddi cells in culture
摘要
Abstract
<正> Objective: To discuss the relationship between hypercholesterolemic disease and the functional and structural changes of Sphincter of Oddi (SO) by the study of effect of Cholesterol Liposome (CL) on structural and quantitative changes of SO cells. Methods: Rabbit SO was isolated for primary cell culture and subculture. After subcultured with different concentration of CL culture medium for 20 h
the structural and quantitative changes of SO cells were analyzed and detected by MTT-test
flow cytometer (FCM)
electronic microscope and electrophoresis technique respectively. Results: CL contributed a prominent stimulus to SO cells proliferation at middle concentration (<0. 5 - 0. 8 mg/ml)
which could be confirmed by FCM analysis which indicated the number of SO cells in S-phase increasing remarkably; however
high concentration of CL inhibited SO cells’ proliferation (>1. 0 mg/ml) and induced apoptosis of SO cells. Swelled mitochondria and dilated endoplasmic reticulum as well as disjoined and diminished
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