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大鼠角质形成细胞培养方法的进一步优化:葡萄糖和氯化钠的滴定

Further optimization of culture method for rat keratinocytes: titration of glucose and sodium chloride.

作者信息

Oku H, Yamashita M, Iwasaki H, Chinen I

机构信息

Laboratory of Applied Biochemistry, Faculty of Agriculture, University of The Ryukyus, Okinawa-Ken, Japan.

出版信息

In Vitro Cell Dev Biol Anim. 1999 Feb;35(2):67-74. doi: 10.1007/s11626-999-0003-y.

Abstract

The present study further improved the serum-free method of culturing rat keratinocytes. To obtain the best growth of rat keratinocytes, we modified our previous serum-free medium (MCDB153 based medium), particularly the amounts of glucose and sodium chloride (NaCl). Titration experiments showed the optimal concentration to be 0.8 mM for glucose and 100 mM for NaCl. This modification eliminated the requirement for albumin, which had been essential for colony formation when our previous medium was used. Titration of glucose and NaCl, followed by adjustment of essential amino acids and growth factors, produced a new formulation. More satisfactory and better growth was achieved with the new medium than with the previous medium. Accumulation of monoalkyldiacylglycerol (MADAG) was consistently noted in this study, representing the unusual lipid profile. A tendency toward normalization was, however, noted with the neutral lipid profile of keratinocytes cultivated in the new medium: lower production of MADAG was obtained with the new formulation, rather than the previous one.

摘要

本研究进一步改进了大鼠角质形成细胞的无血清培养方法。为使大鼠角质形成细胞实现最佳生长,我们对先前的无血清培养基(基于MCDB153的培养基)进行了改良,特别是葡萄糖和氯化钠(NaCl)的用量。滴定实验表明,葡萄糖的最佳浓度为0.8 mM,氯化钠的最佳浓度为100 mM。这种改良消除了对白蛋白的需求,而在使用先前的培养基时,白蛋白对集落形成至关重要。对葡萄糖和氯化钠进行滴定,随后调整必需氨基酸和生长因子,得出了一种新配方。与先前的培养基相比,新培养基实现了更令人满意且更好的生长。在本研究中持续观察到单烷基二酰甘油(MADAG)的积累,这代表了异常的脂质谱。然而,在新培养基中培养的角质形成细胞的中性脂质谱有趋于正常化的趋势:新配方产生的MADAG产量低于先前配方。

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