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在滚筒培养和斯托皮尼共培养中,植入的胚胎感觉神经元将轴突投射向成年听觉脑干神经元。

Implanted embryonic sensory neurons project axons toward adult auditory brainstem neurons in roller drum and Stoppini co-cultures.

作者信息

Thonabulsombat Charoensri, Johansson Saga, Spenger Christian, Ulfendahl Mats, Olivius Petri

机构信息

Department of Anatomy, Faculty of Science, Bangkok 10400& Institute of Science and Technology for Research and Development, Mahidol University, Salaya, Phutthamonthon, Nakorn Pathom 73170, Thailand.

出版信息

Brain Res. 2007 Sep 19;1170:48-58. doi: 10.1016/j.brainres.2007.06.085. Epub 2007 Jul 27.

DOI:10.1016/j.brainres.2007.06.085
PMID:17716633
Abstract

Previously we have shown in vivo the survival, migration and integration of embryonic dorsal root ganglion (DRG) neurons that were grafted into the inner ear and peripheral auditory nervous system. In order to evaluate relevant factors determining integration of sensory neurons further into the central auditory nervous system, complementary in vitro techniques are necessary. The advantages of in vitro systems are that a large number of factors including various grafts and different conditions can be efficiently examined for. Hence, we co-cultured 300 microm thick postnatal rat brainstem slices containing the cochlear nucleus including the central part of the 8th cranial nerve with mouse embryonic DRG neurons. The organotypic co-cultures were either grown on coverslips using the roller drum method described by Gähwiler or on membranes according to the interface method described by Stoppini. Neurons in the cochlear nucleus were labeled with DiI. The results demonstrate that (1) brainstem slices survive for up to 5 weeks in culture, and that (2) co-cultures of embryonic sensory neurons and brainstem show a high degree of neuronal survival, and that (3) survival and axonal outgrowth from the implanted embryonic neurons are dependent on the presence of the brainstem slice rather than on exogenous NGF and that (4) implanted embryonic neurons send axons toward neurons in the cochlear nucleus.

摘要

此前我们已经在体内证明了移植到内耳和外周听觉神经系统的胚胎背根神经节(DRG)神经元的存活、迁移和整合。为了进一步评估决定感觉神经元整合到中枢听觉神经系统的相关因素,需要补充体外技术。体外系统的优点是可以有效地检测大量因素,包括各种移植物和不同条件。因此,我们将包含耳蜗核(包括第8对脑神经的中央部分)的300微米厚的新生大鼠脑干切片与小鼠胚胎DRG神经元进行了共培养。器官型共培养物要么使用Gähwiler描述的滚筒法在盖玻片上生长,要么根据Stoppini描述的界面法在膜上生长。耳蜗核中的神经元用DiI标记。结果表明:(1)脑干切片在培养中存活长达5周;(2)胚胎感觉神经元与脑干的共培养显示出高度的神经元存活;(3)植入的胚胎神经元的存活和轴突生长依赖于脑干切片的存在,而不是外源性NGF;(4)植入的胚胎神经元向耳蜗核中的神经元发出轴突。

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