Abstract

Membrane transport of Cl has an important role in cellular regulatory, absorptive and secretory processes. The techniques presently in use for measurement of Cl transport, including patch-clamp, microelectrodes and 36C1 tracer methods, have restricted sensitivities, time resolution and applicability. Based on the utility of fluorescence probes in examining physiological questions (fluoresceins to study pH, fura-2 to study Ca), we have been developing new fluorescence methods to study Cl transport in membrane vesicles, cells and intact epithelia. We have found that the fluorescence of several quinolinium derivatives is Cl-sensitive and specific and responds rapidly to changes in (C1). The probes can be loaded non-invasively into vesicles and cells to provide a continuous record of (C1).
The aims of this grant request are: to optimize the chemical structure of the Cl indicator for use in measurement of cell (C1), to characterize the best Cl indicators to provide a prescription for their use in physiological measurements, and to use Cl indicators to characterize mechanisms of proximal tubule Cl transport. Using well-established methods in synthetic organic chemistry, the structure of the Cl indicator will be modified to maximize sensitivity, to optimize cell loading and trapping, and to produce the most favorable fluorescent properties including a wavelength shift in the emission spectrum with changes in (C1). Probes will be characterized in terms of their Cl sensitivity, specificity, response time, cell loading, toxicity and intracellular calibration. Mechanisms of Cl transport will be examined in isolated brush border and basolateral membrane vesicles from the renal proximal tubule, in isolate proximal tubule cells and in the intact proximal tubule. Cuvette fluorimetry and fluorescence microscopy will be used. The availability of a good fluorescent Cl indicator should have wide applications in transport physiology and facilitate the understanding of Cl transport mechanisms and Cl regulation in both epithelial and non-epithelial membranes.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK039354-04
Application #
3239188
Study Section
Physiology Study Section (PHY)
Project Start
1988-04-01
Project End
1992-03-31
Budget Start
1991-04-01
Budget End
1992-03-31
Support Year
4
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Type
Schools of Medicine
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Emans, N; Verkman, A S (1996) Real-time fluorescence measurement of cell-free endosome fusion: regulation by second messengers. Biophys J 71:487-94
Periasamy, N; Verkman, A S (1992) Subtraction of background fluorescence in multiharmonic frequency-domain fluorimetry. Anal Biochem 201:107-13
Verkman, A S; Chao, A C; Hartmann, T (1992) Hormonal regulation of Cl transport in polar airway epithelia measured by a fluorescent indicator. Am J Physiol 262:C23-31
Reenstra, W W; Sabolic, I; Bae, H R et al. (1992) Protein kinase A dependent membrane protein phosphorylation and chloride conductance in endosomal vesicles from kidney cortex. Biochemistry 31:175-81
Hartmann, T; Verkman, A S (1992) Construction and performance of a rapid scan monochromator for multiwavelength fluorimetry. Anal Biochem 200:139-42
Biwersi, J; Farah, N; Wang, Y X et al. (1992) Synthesis of cell-impermeable Cl-sensitive fluorescent indicators with improved sensitivity and optical properties. Am J Physiol 262:C242-50
Echevarria, M; Verkman, A S (1992) Optical measurement of osmotic water transport in cultured cells. Role of glucose transporters. J Gen Physiol 99:573-89
Zen, K; Biwersi, J; Periasamy, N et al. (1992) Second messengers regulate endosomal acidification in Swiss 3T3 fibroblasts. J Cell Biol 119:99-110
Zhang, R; Alper, S L; Thorens, B et al. (1991) Evidence from oocyte expression that the erythrocyte water channel is distinct from band 3 and the glucose transporter. J Clin Invest 88:1553-8
Shi, L B; Fushimi, K; Verkman, A S (1991) Solvent drag measurement of transcellular and basolateral membrane NaCl reflection coefficient in kidney proximal tubule. J Gen Physiol 98:379-98

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