用荧光指示剂呋喃甲酰三氟丙酮监测完整青蛙骨骼肌纤维中的肌质钙瞬变。
Myoplasmic calcium transients in intact frog skeletal muscle fibers monitored with the fluorescent indicator furaptra.
作者信息
Konishi M, Hollingworth S, Harkins A B, Baylor S M
机构信息
Department of Physiology, University of Pennsylvania Medical Center, Philadelphia 19104-6085.
出版信息
J Gen Physiol. 1991 Feb;97(2):271-301. doi: 10.1085/jgp.97.2.271.
Furaptra (Raju, B., E. Murphy, L. A. Levy, R. D. Hall, and R. E. London. 1989. Am. J. Physiol. 256:C540-C548) is a "tri-carboxylate" fluorescent indicator with a chromophore group similar to that of fura-2 (Grynkiewicz, G., M. Poenie, and R. Y. Tsien. 1985. J. Biol. Chem. 260:3440-3450). In vitro calibrations indicate that furaptra reacts with Ca2+ and Mg2+ with 1:1 stoichiometry, with dissociation constants of 44 microM and 5.3 mM, respectively (16-17 degrees C; ionic strength, 0.15 M; pH, 7.0). Thus, in a frog skeletal muscle fiber stimulated electrically, the indicator is expected to respond to the change in myoplasmic free [Ca2+] (delta[Ca2+]) with little interference from changes in myoplasmic free [Mg2+]. The apparent longitudinal diffusion constant of furaptra in myoplasm was found to be 0.68 (+/- 0.02, SEM) x 10(-6) cm2 s-1 (16-16.5 degrees C), a value which suggests that about half of the indicator was bound to myoplasmic constituents of large molecular weight. Muscle membranes (surface and/or transverse-tubular) appear to have some permeability to furaptra, as the total quantity of indicator contained within a fiber decreased after injection; the average time constant of the loss was 302 (+/- 145, SEM) min. In fibers containing less than 0.5 mM furaptra and stimulated by a single action potential, the calibrated peak value of delta[Ca2+] averaged 5.1 (+/- 0.3, SEM) microM. This value is about half that reported in the preceding paper (9.4 microM; Konishi, M., and S. M. Baylor. 1991. J. Gen. Physiol. 97:245-270) for fibers injected with purpurate-diacetic acid (PDAA). The latter difference may be explained, at least in part, by the likelihood that the effective dissociation constant of furaptra for Ca2+ is larger in vivo than in vitro, owing to the binding of the indicator to myoplasmic constituents. The time course of furaptra's delta[Ca2+], with average values (+/- SEM) for time to peak and half-width of 6.3 (+/- 0.1) and 9.5 (+/- 0.4) ms, respectively, is very similar to that of delta[Ca2+] recorded with PDAA. Since furaptra's delta[Ca2+] can be recorded at a single excitation wavelength (e.g., 420 nm) with little interference from fiber intrinsic changes, movement artifacts, or delta[Mg2+], furaptra represents a useful myoplasmic Ca2+ indicator, with properties complementary to those of other available indicators.
呋喃普拉特拉(拉朱,B.,E. 墨菲,L. A. 利维,R. D. 霍尔,以及R. E. 伦敦。1989年。《美国生理学杂志》256卷:C540 - C548页)是一种“三羧酸盐”荧光指示剂,其发色团基团与呋喃 - 2(格林基维茨,G.,M. 波涅,以及R. Y. 钱恩。1985年。《生物化学杂志》260卷:3440 - 3450页)的相似。体外校准表明,呋喃普拉特拉与Ca²⁺和Mg²⁺以1:1的化学计量比反应,解离常数分别为44微摩尔和5.3毫摩尔(16 - 17摄氏度;离子强度,0.15摩尔;pH值,7.0)。因此,在电刺激的青蛙骨骼肌纤维中,预计该指示剂对肌浆游离[Ca²⁺](Δ[Ca²⁺])的变化做出反应,而受肌浆游离[Mg²⁺]变化的干扰很小。发现呋喃普拉特拉在肌浆中的表观纵向扩散常数为0.68(±0.02,标准误)×10⁻⁶平方厘米·秒⁻¹(16 - 16.5摄氏度),该值表明约一半的指示剂与大分子质量的肌浆成分结合。肌肉膜(表面和/或横管)似乎对呋喃普拉特拉有一定通透性,因为注射后纤维内所含指示剂的总量减少;损失的平均时间常数为302(±145,标准误)分钟。在含有低于0.5毫摩尔呋喃普拉特拉且由单个动作电位刺激的纤维中,校准后的Δ[Ca²⁺]峰值平均值为5.1(±0.3,标准误)微摩尔。该值约为前一篇论文(9.4微摩尔;小西,M.,以及S. M. 贝勒。1991年。《普通生理学杂志》97卷:245 - 270页)中报道的注射紫尿酸二乙酸(PDAA)的纤维的一半。后一种差异至少部分可以解释为,由于指示剂与肌浆成分结合,呋喃普拉特拉对Ca²⁺的有效解离常数在体内可能比体外更大。呋喃普拉特拉的Δ[Ca²⁺]的时间进程,达到峰值的时间和半高宽的平均值(±标准误)分别为6.3(±0.1)和9.5(±0.4)毫秒,与用PDAA记录的Δ[Ca²⁺]非常相似。由于呋喃普拉特拉的Δ[Ca²⁺]可以在单个激发波长(例如420纳米)下记录,几乎不受纤维固有变化、运动伪迹或Δ[Mg²⁺]的干扰,呋喃普拉特拉是一种有用的肌浆Ca²⁺指示剂,其特性与其他现有指示剂互补。
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