Measurement of the cytosolic free calcium ion concentration of individual lymphocytes by microfluorometry using quin 2 or fura-2.
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- Komada Hiroshi
- Microbiology Mie University School of Medicine
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- Nakabayashi Hiroshi
- Departments of Patholoky Mie University School of Medicine
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- Yoshida Toshimichi
- Departments of Patholoky Mie University School of Medicine
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- Takanari Hideki
- Departments of Patholoky Mie University School of Medicine
Description
The cytosolic free calcium ion concentration ([Ca2+]i) of individual lymphocytes was measured by microfluorometry with dual excitation wavelengths using quin 2 or fura-2. Fura-2 was a more suitable fluorescent Ca2+ indicator than quin 2 for measurements of single cells because the standard curve calibrated for fura-2 had a good linearity, and the standard deviation (SD) of the value of the intensity ratio of fura-2-loaded cells was much smaller than that of quin 2-loaded cells. The [Ca2+]i in quiescent lymphocytes was about 1 x 10-7 M, and an increase in the [Ca2+]i was observed within a few minutes of ionomycin, protein A, phorbol myristate acetate (PMA) or concanavalin A (Con A) stimulation. Ionomycin-induced proliferation occurred when the initial [Ca2+]i was approximately 3 x 10-7 M or greater. The increase in the [Ca2+]i induced by Con A occurred transiently, and another rise in the [Ca2+]i was observed in the stage prior to the S-phase. These results indicate that Ca2+ is necessary for stimulated lymphocytes to enter the cell cycle and S-phase.
Journal
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- Cell Structure and Function
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Cell Structure and Function 14 (2), 141-150, 1989
Japan Society for Cell Biology
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Details 詳細情報について
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- CRID
- 1390282679670871552
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- NII Article ID
- 130003512605
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- COI
- 1:CAS:528:DyaL1MXltlSjt7Y%3D
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- ISSN
- 13473700
- 03867196
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- PubMed
- 2743418
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- Text Lang
- en
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- Article Type
- journal article
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- Data Source
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- JaLC
- Crossref
- PubMed
- CiNii Articles
- OpenAIRE
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- Abstract License Flag
- Disallowed
