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虎螈视网膜视杆细胞外段的钙稳态

Calcium homeostasis in the outer segments of retinal rods from the tiger salamander.

作者信息

Lagnado L, Cervetto L, McNaughton P A

机构信息

Physiological Laboratory, Cambridge.

出版信息

J Physiol. 1992 Sep;455:111-42. doi: 10.1113/jphysiol.1992.sp019293.

Abstract
  1. The processes regulating intracellular calcium in the outer segments of salamander rods have been investigated. The main preparation used was the isolated rod loaded with the Ca(2+)-sensitive photoprotein aequorin, from which outer segment membrane current and free [Ca2+]i could be recorded simultaneously. Two other preparations were also used: outer segment membrane current was recorded from intact, isolated rods using a suction pipette, and from detached outer segments using a whole-cell pipette. 2. Measurements of free intracellular [Ca2+] in Ringer solution were obtained from two aequorin-loaded rods. Mean [Ca2+]i in darkness was 0.41 microM, and after a bright flash [Ca2+]i fell to below detectable levels ( < 0.3 microM). No release of intracellular Ca2+ by a bright flash of light could be detected ( < 0.2 microM). 3. Application of the phosphodiesterase inhibitor 3-isobutyl-1-methylxanthine (IBMX) caused an increase in the size of the light-sensitive current and a rise in [Ca2+]i, but application of IBMX either when the light-sensitive channels had been closed by a bright light or in the absence of external Ca2+ caused no detectable rise in [Ca2+]i. It is concluded that IBMX increases [Ca2+]i by opening light-sensitive channels, and does not release Ca2+ from stores within the outer segment. 4. Removal of external Na+ caused a rise in [Ca2+]i to around 2 microM and completely suppressed the light-sensitive current. 5. The Na(+)-Ca2+, K+ exchange current in aequorin-loaded rods was activated in first-order manner by internal free calcium, with a mean Michaelis constant, KCa, of 1.6 microM. 6. The KCa of the Na(+)-Ca2+, K+ exchange was increased by elevating internal [Na+]. 7. The Michaelis relation between [Ca2+]i and the activity of the Na(+)-Ca2+, K+ exchange was used to calculate the change in [Ca2+]i occurring during the response to a bright light. In aequorin-loaded rods in Ringer solution the mean change in free [Ca2+]i after a bright flash was 0.34 microM. In these rods 10% of the dark current was carried by Ca2+. 8. Most of the calcium entering the outer segment was taken up rapidly and reversibly by buffer systems. The time constant of equilibration between free and rapidly bound Ca2+ was less than 20 ms. No slow component of calcium uptake was detected. 9. Two components of calcium buffering could be distinguished in the outer segments of aequorin-loaded rods.(ABSTRACT TRUNCATED AT 400 WORDS)
摘要
  1. 对蝾螈视杆细胞外段调节细胞内钙的过程进行了研究。主要使用的制备方法是将分离的视杆细胞装载对Ca(2+)敏感的光蛋白水母发光蛋白,由此可同时记录外段膜电流和游离的[Ca2+]i。还使用了另外两种制备方法:用吸管从完整分离的视杆细胞记录外段膜电流,用全细胞膜片钳从分离的外段记录膜电流。2. 从两个装载了水母发光蛋白的视杆细胞中获取了林格氏液中细胞内游离[Ca2+]的测量值。黑暗中平均[Ca2+]i为0.41微摩尔,强光闪光后[Ca2+]i降至可检测水平以下(<0.3微摩尔)。未检测到强光闪光引起的细胞内Ca2+释放(<0.2微摩尔)。3. 应用磷酸二酯酶抑制剂3 - 异丁基 - 1 - 甲基黄嘌呤(IBMX)导致光敏感电流大小增加以及[Ca2+]i升高,但在强光使光敏感通道关闭时或无细胞外Ca2+存在时应用IBMX,未检测到[Ca2+]i有可检测到的升高。得出的结论是,IBMX通过打开光敏感通道增加[Ca2+]i,而不是从外段内的储存库中释放Ca2+。4. 去除细胞外Na+导致[Ca2+]i升高至约2微摩尔,并完全抑制了光敏感电流。5. 装载了水母发光蛋白的视杆细胞中的Na(+)-Ca2+、K+交换电流以一级方式被细胞内游离钙激活,平均米氏常数KCa为1.6微摩尔。6. 通过提高细胞内[Na+],Na(+)-Ca2+、K+交换的KCa增加。7. [Ca2+]i与Na(+)-Ca2+、K+交换活性之间的米氏关系用于计算强光响应过程中发生的[Ca2+]i变化。在林格氏液中装载了水母发光蛋白的视杆细胞中,强光闪光后游离[Ca2+]i的平均变化为0.34微摩尔。在这些视杆细胞中,10%的暗电流由Ca2+携带。8. 进入外段的大部分钙被缓冲系统快速且可逆地摄取。游离钙与快速结合钙之间平衡的时间常数小于20毫秒。未检测到钙摄取的慢成分。9. 在装载了水母发光蛋白的视杆细胞外段中可区分出两种钙缓冲成分。(摘要截断于400字)

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