综合图区亚洲网友自拍|亚洲黄色网络|成人无码网WWW在线观看,日本高清视频色视频kk266,激情综合五月天,欧美一区日韩一区中文字幕页

English | 中文版 | 手機版 企業(yè)登錄 | 個人登錄 | 郵件訂閱
當前位置 > 首頁 > 技術(shù)文章 > Isolation and culture of smooth muscle cell

Isolation and culture of smooth muscle cell

瀏覽次數(shù):2216 發(fā)布日期:2017-3-16  來源:本站 僅供參考,謝絕轉(zhuǎn)載,否則責任自負

1.Male Wistar rats of about 250g body wt were anesthetized with ether and were decapitated.
 
2.Kidneys and thoracic aorta were removed, rinsed with sterile ice-cold phosphate-buffered saline (PBS; 1.5 mmol/L KH2PO4, 2.7 mmol/L Na2HPO4, 153.8 mmol/L NaCl), and placed in PBS on ice.  If renal vascular trees were isolated for cell culture, the following steps were carried out under a laminar flow hood obeying sterile conditions.
 
3.After complete and deep resection of the renal artery, kidneys were decapsulated and longitudinally bisected, and the medullae were removed.

4.Kidney halves were pressed with their surface against stainless steel grids of 40 and 50 mesh size (420 and 300 m openings, respectively).
 
5.Renal vascular trees were gently rubbed against the grids and washed with cold isotonic saline.
 
6.The optimal force, which was exerted on the vessels, represented a compromise between purity and viability, corresponding to high and low force, respectively.
 
7.By this procedure, renal parenchyma passed through the meshes, while entire renal vascular trees were retained on the grid and could be picked up with fine forceps.
 
8.Finally, renal vascular trees were extensively washed on a grid of 150 mesh size (100 m openings) with a jet stream of cold isotonic saline.
 
9.Renal vascular trees were treated with collagenase and transferred into 25 cm2 culture flasks, which contained 1 mL Dulbecco's modified Eagle medium (DMEM) supplemented with 20% fetal bovine serum (FBS), penicillin (100U/mL), and streptomycin (0.1 mg/mL).
 
10.Culture flasks were coated with collagen type I from rat tail to prevent floating of explants.
 
11.Culture flasks were incubated at 37°C in a humidified atmosphere of 10% CO2 in air.
 
12.Medium volume was increased as soon as the explants were firmly attached.
 
13.Explants were removed from the culture flasks about 10 to 14 days later, when a sufficient amount of cells had grown out. After two to three weeks, cells were subcultured by trypsinization.
 
14.Cells were passaged as they became confluent and were diluted 1:5.
 
15.After the first subculture, cells were grown in antibiotic-free medium, consisting of DMEM supplemented with 20% FBS.
 
16.The medium was exchanged every two days.

來源:武漢原生原代生物醫(yī)藥科技有限公司
聯(lián)系電話:027-87490190
E-mail:service@pricells.com.cn

用戶名: 密碼: 匿名 快速注冊 忘記密碼
評論只代表網(wǎng)友觀點,不代表本站觀點。 請輸入驗證碼: 8795
Copyright(C) 1998-2024 生物器材網(wǎng) 電話:021-64166852;13621656896 E-mail:info@bio-equip.com