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Synaptic calcium 2+ and information coding in vertebrate rods and cones.

机译:突触钙2+和脊椎动物杆和视锥细胞中的信息编码。

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摘要

Rod and cone photoreceptors encode light with different sensitivity and kinetics. Here we use optical imaging method to study the synaptic differences that affect the transmission of visual information. We find that rods tonically release synaptic vesicles in the dark at a much slower rate than cones, as measured by the release of the fluorescent vesicle indicator FMI-43. Rods signal under dimmer light, which has a lower signal-to-noise ratio than bright light. The slower release from rods matches the precision signal output to the information content of light input, which optimizes use of the limited resource of continuously cycling vesicles. To elucidate the mechanism underlying slower release from rods, we evaluate Ca2+-dependent release by simultaneously recording synaptic vesicle cycling and intraterminal Ca2+. We find that the Ca2+ sensitivity of release is indistinguishable in rods and cones, consistent with their possessing similar release machinery. However, we find the dark intraterminal Ca2+ concentration is lower in rods than in cones, as determined by 2-photon Ca 2+ imaging. Thus, the lower level of dark Ca2+ ensures that rods encode intensity with a slower vesicle release rate that is better matched to the lower information content of dim light.
机译:杆和锥光感受器编码具有不同灵敏度和动力学的光。在这里,我们使用光学成像方法来研究影响视觉信息传递的突触差异。我们发现杆状体在黑暗中以比锥状体慢得多的速率在黑暗中音调释放突触囊泡,如荧光囊泡指示剂FMI-43的释放所测量。杆在较暗的光线下发出信号,该信号的信噪比低于明亮的光线。从杆释放的速度较慢,将精确的信号输出与光输入的信息内容相匹配,从而优化了有限的连续循环囊泡资源的使用。为了阐明从杆中缓慢释放的机制,我们通过同时记录突触小泡循环和末端内Ca2 +来评估Ca2 +依赖性释放。我们发现,Ca2 +的释放敏感性在棒和锥中是无法区分的,这与它们具有类似的释放机制是一致的。但是,我们发现,通过2光子Ca 2+成像确定,杆中暗的末端Ca2 +浓度低于视锥中的浓度。因此,较低水平的深色Ca2 +可确保棒以较低的囊泡释放速率编码强度,从而更好地与较低的暗光信息含量匹配。

著录项

  • 作者

    Sheng, Zejuan.;

  • 作者单位

    University of California, Berkeley.;

  • 授予单位 University of California, Berkeley.;
  • 学科 Biology Neuroscience.
  • 学位 Ph.D.
  • 年度 2007
  • 页码 128 p.
  • 总页数 128
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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