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Caged compounds for multichromic optical interrogation of neural systems

机译:笼状化合物用于神经系统的多色光学询问

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摘要

Caged compounds have widely used by neurophysiologists to study many aspects of cellular signaling in glia and neurons. Biologically inert before irradiation, they can be loaded into cells via patch pipette or topically applied in situ to a defined concentration, photolysis releases the caged compound in a very rapid and spatially defined way. Since caged compounds are exogenous optical probes, they include not only natural products such neurotransmitters, calcium and IP3, but non-natural products such as fluorophores, drugs and antibodies. In this Technical Spotlight we provide a short introduction to the uncaging technique by discussing the nitroaromatic caging chromophores most widely used in such experiments (e.g. CNB, DMNB, MNI and CDNI). We show that recently developed caging chromophores (RuBi and DEAC450) that are photolyzed with blue light (ca. 430–480 nm range) can be combined with traditional nitroaromatic caged compounds to enable two-color optical probing of neuronal function. For example, one-photon uncaging of either RuBi-GABA or DEAC450-GABA with a 473-nm laser is facile, and can block non-linear currents (dendritic spikes or action potentials) evoked by two-photon uncaging of CDNI-Glu at 720 nm. We also show that two-photon uncaging of DEAC450-Glu and CDNI-GABA at 900 and 720 nm, respectively, can be used to fire and block action potentials. Our experiments illustrate that recently developed chromophores have taken uncaging out of the “monochrome era”, in which it has existed since 1978, so as to enable multichromic interrogation of neuronal function with single synapse precision.
机译:笼状化合物已被神经生理学家广泛用于研究神经胶质细胞和神经元中细胞信号传导的许多方面。辐照前具有生物惰性,可以通过贴片移液器将其加载到细胞中,或以一定浓度就地局部应用,光解以非常快速和空间限定的方式释放笼状化合物。由于笼状化合物是外源性光学探针,因此它们不仅包括天然产物,例如神经递质,钙和IP3,还包括非天然产物,例如荧光团,药物和抗体。在本技术聚焦中,我们通过讨论在此类实验中最广泛使用的硝基芳族笼型生色团(例如CNB ,DMNB,MNI和CDNI)来简要介绍开壳技术。我们显示,最近开发的笼状生色团(RuBi和DEAC450)可以被蓝光(约430–480 nm范围)光解,可以与传统的硝基芳族笼状化合物结合使用,以实现神经功能的双色光学探测。例如,使用473 nm激光对RuBi-GABA或DEAC450-GABA进行单光子解囊是很容易的,并且可以阻止CDNI-Glu的两光子解笼引起的非线性电流(树突状峰或动作电位)。 720纳米我们还显示DEAC450-Glu和CDNI-GABA分别在900 nm和720 nm处的双光子解笼可用于激发和阻断动作电位。我们的实验表明,最近开发的发色团已经摆脱了自1978年就已经存在的“单色时代”,从而能够以单个突触精度对神经元功能进行多色询问。

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