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利用双光子激发对飞升体积内的笼形钙进行光解。

Photolysis of caged calcium in femtoliter volumes using two-photon excitation.

作者信息

Brown E B, Shear J B, Adams S R, Tsien R Y, Webb W W

机构信息

Developmental Resource for Biophysical Imaging and Optoelectronics, Cornell University, Ithaca, New York 14853, USA.

出版信息

Biophys J. 1999 Jan;76(1 Pt 1):489-99. doi: 10.1016/S0006-3495(99)77217-6.

Abstract

A new technique for the determination of the two-photon uncaging action cross section (deltau) of photolyzable calcium cages is described. This technique is potentially applicable to other caged species that can be chelated by a fluorescent indicator dye, as well as caged fluorescent compounds. The two-photon action cross sections of three calcium cages, DM-nitrophen, NP-EGTA, and azid-1, are studied in the range of excitation wavelengths between 700 and 800 nm. Azid-1 has a maximum deltau of approximately 1.4 GM at 700 nm, DM-nitrophen has a maximum deltau of approximately 0.013 GM at 730 nm, and NP-EGTA has no measurable uncaging yield. The equations necessary to predict the amount of cage photolyzed and the temporal behavior of the liberated calcium distribution under a variety of conditions are derived. These equations predict that by using 700-nm light from a Ti:sapphire laser focused with a 1.3-NA objective, essentially all of the azid-1 within the two-photon focal volume would be photolyzed with a 10-micros pulse train of approximately 7 mW average power. The initially localized distributions of free calcium will dissipate rapidly because of diffusion of free calcium and uptake by buffers. In buffer-free cytoplasm, the elevation of the calcium concentration at the center of the focal volume is expected to last for approximately 165 micros.

摘要

描述了一种用于测定可光解钙笼的双光子解笼作用截面(δu)的新技术。该技术可能适用于其他可被荧光指示剂染料螯合的笼状物质,以及笼状荧光化合物。在700至800nm的激发波长范围内研究了三种钙笼DM - 硝基苯酚、NP - EGTA和叠氮 - 1的双光子作用截面。叠氮 - 1在700nm处的最大δu约为1.4 GM,DM - 硝基苯酚在730nm处的最大δu约为0.013 GM,而NP - EGTA没有可测量的解笼产率。推导了预测在各种条件下笼状物质光解量和释放钙分布的时间行为所需的方程。这些方程预测,通过使用来自钛宝石激光器的700nm光,用1.3 - NA物镜聚焦,在双光子焦体积内基本上所有的叠氮 - 1将被平均功率约为7 mW的10微秒脉冲序列光解。由于游离钙的扩散和缓冲剂的摄取,游离钙最初的局部分布将迅速消散。在无缓冲剂的细胞质中,预计焦体积中心的钙浓度升高将持续约165微秒。

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