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[通过经心脏插管逆行肝脏灌注法分离小鼠原代肝细胞]

[Isolation of mouse primary hepatocytes by retrograde liver perfusion with catheterization via heart].

作者信息

Bai Yan-Nan, Zhang Tao, Wu Hong, Zeng Yong

机构信息

Department of Hepato-Biliary-Pancreatic Surgery, West China Hospital, Sichuan University, Chengdu 610041, China.

出版信息

Sichuan Da Xue Xue Bao Yi Xue Ban. 2014 Jan;45(1):138-41.

Abstract

OBJECTIVE

To explore the effects of retrograde liver perfusion with catheterization via heart on the isolation of primary mouse hepatocytes.

METHODS

In order to more efficiently isolate primary mouse hepatocytes, we improved the traditional two-step collagenase perfusion method. The liver perfusion catheter was inserted through right atrium and suprahepatic vena cava, and the perfusion velocity was controlled by the drip infusion with collagenase perfusate containing 10% of fetal calf serum.

RESULTS

Total success rate of catheterization in the improved group was as high as 95%, and the success rate of first at ttempt in the improved group was significantly higher than that in the traditional group (94.7% vs. 68.8%). Liver perfusion in the improved group was symmetrical with the high yield of hepatocytes up to 1.07 x 10(6) per gram of mouse weight and 92.16% of average cell vitality, which were higher than those in the traditional group.

CONCLUSION

The retrograde liver perfusion through the heart is a simple and easy-to-learn method to isolate mouse primary hepatocytes, which also could guarantee the satisfactory yield and vitality of primary hepatocytes.

摘要

目的

探讨经心脏导管逆行肝脏灌注对原代小鼠肝细胞分离的影响。

方法

为了更高效地分离原代小鼠肝细胞,我们改进了传统的两步胶原酶灌注法。将肝脏灌注导管经右心房和肝上腔静脉插入,通过滴注含10%胎牛血清的胶原酶灌注液来控制灌注速度。

结果

改进组导管插入的总成功率高达95%,改进组首次尝试的成功率显著高于传统组(94.7%对68.8%)。改进组肝脏灌注均匀,每克小鼠体重肝细胞产量高达1.07×10⁶个,平均细胞活力为92.16%,均高于传统组。

结论

经心脏逆行肝脏灌注是一种简单易学的分离小鼠原代肝细胞的方法,还能保证原代肝细胞令人满意的产量和活力。

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