人毛囊单位体外保存培养研究

目的通过对不同保存培养液下毛囊单位生长情况的研究，旨在寻找一种更为适合的毛囊保存培养液。方法：将添加不同配方的毛囊培养液进行毛囊培养，观察并计算毛囊生长长度。结果：本研究中⑤的保存培养液提高了毛囊单位的成活率，毛囊单位的生长速度明显加快，平均生长天数延长至14 d以上，最终生长长度可达（1．075±O．215）mm。结论：本研究中⑤的保存培养液有利于毛囊的持续、稳定生长延长，并对局部受损毛囊的增值再生具有促进作用，效果良好，明显优于传统培液。

Preparation, cryopreservation and in vitro culture of spermatogonial stem cells of new born calves

The experiment was designed to study the preparation, cryopreservation and culture of calf spermatogonial stem cells in order to provide some data for theoretical research and practical use of calf spermatogonial stem cells. As for enzymolysis of testis tissue, two digestive method A and B. The cryopreservation cooling procedure was that spermatogonial stem cells was equilibrated at 4℃ for lh, at -20℃ for lh, at -40℃ for 2h, at -80℃ overnight and then stored in liquid nitrogen. The different concentration of three eryoprotectants were compared. The results indicated that both method A and method B achieved the same high motility rates of cells with method B needing time longer, calf spermatogonial stem cells could be well cryopreserved by the stage cooling procedure. Satisfactory cryopreservative results were gotten by adding 10% DMSO or 10% EG to cryopreservative medium, the former was better and adding sucrose could improved cryopreservative effect. The culture behaviors of spermatogonial stem cells kept the same before and after cryopreservation. It was concluded that an effective method was verified for preparation, cryopreservation and culture of new calf spermatogonial stem cells.