Deprecated: Required parameter $cat_id follows optional parameter $type in /www/wwwroot/ebimall.com/systems/hong.php on line 2088

Deprecated: Required parameter $where follows optional parameter $tree_id in /www/wwwroot/ebimall.com/systems/hlb.php on line 3505
Sphingomyelin Mass Measurement188bio精品生物—专注于实验室精品爆款的电商平台 - 蚂蚁淘旗下精选188款生物医学科研用品
您好,欢迎您进入188进口试剂采购网网站! 服务热线:4000-520-616
蚂蚁淘商城 | 现货促销 | 科研狗 | 生物在线

Sphingomyelin Mass Measurement

Bligh & Dyer extraction1) Pellet approximately 1 X 107 cells.2) Resuspend pellet in 3 ml CHCl3: CH3OH (1:2) and vortex hard.3) Add 0.8 ml H2O, vortex hard and allow solution to sit at room temperature for atleast 30 minutes.4) Pellet cellular debris by spinning at 3,000 rpm (in the tabletop centrifuge) for 5 minutes.5) Transfer solvents to a new tube without transferring any of the pelleted debris.6) Add 1 ml of CHCl3 and 1 ml of H2O to each sample.--> Upon addition of CHCl3, a biphasic solution should result.7) Vortex hard and spin samples at 3,000 rpm (in the tabletop centrifuge) for 5 minutes.8) Remove the upper aqueous/methanolic phase and transfer the lower CHCl3 phase to a new tube.--> The CHCl3 phase should constitute 2 ml total volume.9) Dry down solvent under extra dry nitrogen gas.10) Resuspend lipids in 1 ml of CHCl3, aliquot 800 µl of lipid suspension for base hydrolysis and 100 µl for phosphate measurement.Base hydrolysis9) Bring lipids up to 1 ml volume in CHCl3.10) Add 100 µl of 2N methanolic NaOH to each sample.--> The final concentration of base is 0.2N.11) Incubate samples at 37°C for 1 hour.12) Neutralize base by adding 100 µl of 2N HCl to each sample.13) Add 2 ml CH3OH and 600 µl of water to each sample, vortex hard.14) Allow samples to sit at room temperature for atleast 30 minutes.15) Add 1 ml CHCl3 to break phases and vortex hard.16) Complete the extraction by addition of 1 ml of water, vortex hard.17) Spin samples at 3,000 rpm (in the tabletop centrifuge) for 5 minutes.18) Aspirate off the upper H2O/methanolic phase and collect the lower, CHCl3 phase.19) Dry the lipids down under extra dry nitrogen gas, resuspend them in 75µl of CHCl3 , aliquot 10 µl for phosphate measurements and spot 50µl on a TLC plate.20) Spot standards (1-100 nmoles SM) and develop plates in CHCl3:CH3OH:Acetic acid:H2O (50:30:8:5).21) Visualize lipids using iodine vapor, mark, and scrape the SM spots into a 13x100 screw-capped tube.22) Extract the SM from the silica as follows:a) wash with CHCl3:CH3OH (2:1) 2 timesb) wash with CHCl3:CH3OH (1:2) one time.23) Quantitate the extracted SM via a standard phosphate assay.


新闻动态
行业前沿
技术文章
最新产品

188进口试剂采购网 www.188bio.cn -中国试剂网,试剂网,化学试剂网,国药试剂,抗体公司,试剂公司,试剂盒公司,苏州试剂公司,北京化学试剂公司,天津化学试剂,试剂商城,试剂代理,流式抗体 细胞库查询 sitemap