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一种适用于周围神经组织工程的成年犬雪旺细胞富集和基因改造的新细胞培养方案。

A new cell culture protocol for enrichment and genetic modification of adult canine Schwann cells suitable for peripheral nerve tissue engineering.

作者信息

Haastert K, Seef P, Stein V M, Tipold A, Grothe C

机构信息

Hannover Medical School, Institute of Neuroanatomy, OE 4140 Carl-Neuberg-Str. 1, D-30625 Hannover, Germany.

出版信息

Res Vet Sci. 2009 Aug;87(1):140-2. doi: 10.1016/j.rvsc.2009.01.001. Epub 2009 Feb 18.

Abstract

Easily applicable techniques are presented to obtain high numbers of enriched canine Schwann cells (cSC) in a short time-window. The potential of adult SC for tissue engineering of peripheral nerves and ex vivo gene therapy is obvious from physiological events taking place after peripheral nerve transection [Haastert, K., Grothe, C., 2007. Gene therapy in peripheral nerve reconstruction approaches. Curr. Gene Ther. 7, 221-228]. The presented techniques were modified from a protocol for cultivation and expansion of adult cSC by others [Pauls, J., Nolte, C., Forterre, F., Brunnberg, L., 2004. Cultivation and expansion of canine Schwann cells using reexplantation. Berl. Munch. Tierarztl. Wochenschr. 117, 341-352] and own experiences in rodent and human SC cultivation and transfection [Haastert, K., Mauritz, C., Chaturvedi, S., Grothe, C., 2007. Human and rat adult Schwann cell cultures: fast and efficient enrichment and highly effective non-viral transfection protocol. Nat. Protoc. 2, 99-104]. A purity of about 80% cSC achieved by immunopanning techniques and selective culture conditions is 2.5 fold higher as previously reported (Pauls et al., 2004). Additionally, highly enriched cSC populations are available in 3-4 weeks, only half the time period reported previously (Pauls et al., 2004). Furthermore, electroporation and genetic modification of cSC is reported for the first time.

摘要

本文介绍了一些易于应用的技术,可在短时间内获得大量富集的犬雪旺细胞(cSC)。从周围神经横断后发生的生理事件可以明显看出,成年雪旺细胞在周围神经组织工程和离体基因治疗方面具有潜力[Haastert, K., Grothe, C., 2007. 周围神经重建方法中的基因治疗。《当代基因治疗》7, 221 - 228]。本文介绍的技术是在他人[Pauls, J., Nolte, C., Forterre, F., Brunnberg, L., 2004. 利用再移植培养和扩增犬雪旺细胞。《柏林与慕尼黑兽医周刊》117, 341 - 352]关于成年cSC培养和扩增方案的基础上进行改进,并结合了我们自己在啮齿动物和人类雪旺细胞培养及转染方面的经验[Haastert, K., Mauritz, C., Chaturvedi, S., Grothe, C., 2007. 人和大鼠成年雪旺细胞培养:快速高效的富集及高效非病毒转染方案。《自然实验手册》2, 99 - 104]。通过免疫淘选技术和选择性培养条件获得的约80%纯度的cSC比之前报道的(Pauls等人,2004)高2.5倍。此外,在3 - 4周内即可获得高度富集的cSC群体,仅为之前报道时间(Pauls等人,2004)的一半。此外,首次报道了cSC的电穿孔和基因修饰。

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