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体外化学诱导运动活动后新生大鼠脊髓中硫代罗丹明标记的细胞。

Sulphorhodamine-labelled cells in the neonatal rat spinal cord following chemically induced locomotor activity in vitro.

作者信息

Kjaerulff O, Barajon I, Kiehn O

机构信息

Department of Medical Physiology, Panum Institute, University of Copenhagen, Denmark.

出版信息

J Physiol. 1994 Jul 15;478 ( Pt 2)(Pt 2):265-73. doi: 10.1113/jphysiol.1994.sp020248.

Abstract
  1. Sulphorhodamine 101, a fluorescent dye and newly identified activity marker, was used to localize potential spinal locomotor networks in the neonatal rat spinal cord. 2. Preparations of the spinal cord with one entire hindlimb attached or the spinal cord in isolation were kept in vitro. Spinal locomotor activity was maintained chemically with NMDA (5-7.5 microM), in combination with 5-HT (7.5-20 microM), for 4-4.5 h in the presence of 0.0001-0.0005% sulphorhodamine 101. Matched non-locomoting controls were exposed to the dye in the absence of transmitters for a comparable time. Transverse sections of the lumbar spinal cord (L1-L6) were screened for rhodamine emission using an epifluorescence microscope. 3. In hindlimb-attached locomoting preparations with intact dorsal roots, labelled cells were found on the leg side in the dorsal horn (mainly laminae II-IV), in the intermediate grey (lamina VI-VII) and around the central canal (lamina X). Dorsal rhizotomy was performed on the leg side, to prevent synaptic activity due to afferent inflow. This largely reduced the number of labelled cells in the dorsal horn and in the lateral part of the intermediate grey matter. A further reduction of labelling in these areas was seen after complete isolation of the cord or when compared to the legless side, with the majority of labelled cells persisting in a bilateral cluster close to the central canal and in the medial intermediate grey. Few labelled cells were observed in non-locomoting preparations. The intensity of motoneuronal labelling was variable.(ABSTRACT TRUNCATED AT 250 WORDS)
摘要
  1. 磺基罗丹明101是一种荧光染料,也是新发现的活性标记物,用于定位新生大鼠脊髓中潜在的脊髓运动网络。2. 将附着有一整个后肢的脊髓制剂或孤立的脊髓保存在体外。在存在0.0001 - 0.0005%磺基罗丹明101的情况下,用NMDA(5 - 7.5微摩尔)与5 - HT(7.5 - 20微摩尔)联合化学维持脊髓运动活性4 - 4.5小时。匹配的非运动对照组在无递质的情况下暴露于染料中相同时间。使用落射荧光显微镜筛选腰段脊髓(L1 - L6)的横切片中的罗丹明发射。3. 在背根完整的后肢附着运动制剂中,在背角(主要是II - IV层)、中间灰质(VI - VII层)和中央管周围(X层)的腿部一侧发现了标记细胞。在腿部一侧进行背根切断术,以防止由于传入神经流入引起的突触活动。这在很大程度上减少了背角和中间灰质外侧部分的标记细胞数量。在脊髓完全分离后或与无腿侧相比,这些区域的标记进一步减少,大多数标记细胞持续存在于靠近中央管的双侧簇和内侧中间灰质中。在非运动制剂中观察到的标记细胞很少。运动神经元标记的强度是可变的。(摘要截短于250字)
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/17e0/1155684/5df38143464b/jphysiol00346-0084-a.jpg

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