Photoprotein-mediated measurement of calcium ion concentration in mitochondria of living cells

被引：67

作者：

Rizzuto, R ^{[1
]}

Brini, M ^{[1
]}

Bastianutto, C ^{[1
]}

Marsault, R ^{[1
]}

Pozzan, T ^{[1
]}

机构：

[1] UNIV PADUA,CNR,CTR STUDY BIOMEMBRANES,I-35121 PADUA,ITALY

来源：

MITOCHONDRIAL BIOGENESIS AND GENETICS, PT A | 1995年 / 260卷

关键词：

D O I：

10.1016/0076-6879(95)60155-4

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

This chapter discusses the expression of the transfected complementary DNA (cDNA), the intracellular localization of the recombinant photoprotein, the reconstitution of the active, Ca2+ measuring holoprotein, the measurement of aequorin light emission, and the conversion of luminescence data into estimates of [Ca2+]. It describes the development of a new methodology for measuring [Ca2+]m in living cells. By this approach the chapter demonstrates that the in vivo local domains of [Ca2+]c, sufficiently high to induce fast mitochondrial Ca2+ accumulation, are transiently generated close to plasmalemmal or intracellular Ca2+ channels. Two appealing applications appear to be an important goal for the future: single-cell imaging and the generation of transgenic animals. As to the first, the low-light emission of photoprotein represents a major problem, and work needs to be done, both in the development of suitable apparatus designed for low-light imaging and in the enhancement of the levels of aequorin expression. As to transgenic animals, there is the fascinating possibility of studying mitochondrial Ca2+ homeostasis in situ (e.g., in brain slices). © 1995, Elsevier Inc.

引用

页码：417 / 428

页数：12

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