Abstract

Mesangial cells (MCs) play a critical role in glomerular biology, both in health and disease. The contraction of these vascular-smooth-muscle- like cells is believed to modulate GFR. The proliferation and secretion of matrix substances by MCs plays a central role in the development of many forms of chronic glomerular disease. The regulation of intracellular pH (pHi), important for a wide variety of cellular functions (enzyme activities, ion conductances, etc.), is expected to be especially critical for MCs. That is because both muscle tension and cell proliferation are exquisitely pH sensitive. This proposal is designed to continue an intensive study of the pH (i) physiologies of rat mesangial cells in primary culture (3rd - 8th passage). Our ultimate goal is to understand how pH(i) is regulated in MCs under control conditions, and after short- and long-term exposure to growth factors that act through different signal-transduction pathways. In previous work, we have shown that MCs use three transporters to regulate pH(i): a Na-H exchanger, a Na+-dependent Cl-HCO3 exchanger (both of which cause pH(i) to increase), and a Na+-independent Cl-HCO3 exchanger (which causes pH(i) to decrease). Furthermore, in work on populations of cells, we have shown that (when assayed at a single pH(i) each of these transporters is activated by mitogens, but that the degree of activation is time dependent. Furthermore, we have developed an approach for accurately assessing the effects of mitogens on the pH(i) dependence of the Na-H exchanger. We propose three major aims: First, to characterie the effects of mitogens and cell shrinkage on the pH(i) dependencies of the three transporters. These experiments will be done on populations of MCs loaded with a pH-sensitive fluorescent dye, and studied in a dual- beam spectrofluorometer. Our approach will be to determine the rates of pH(i) recovery from acid or alkali loads, in the absence and presence of specific inhibitors, and use these data to compute the pH(i) dependencies of the fluxes mediated by each of the three transporters. Second, to use a matematical model of pH(i) regulation to determine if the kinetic descriptions of the transporters (derived in the 1st Aim) account for the pH9I0 vs time records (also obtained in the 1st Aim). Third, to determine the long-range effects of mitogens, and the progression to mitosis, on the activities of each of the three transporters. These experiments will be done on multiple individual MCs loaded with a pH- sensitive fluorescent dye, and studied using a microscope-based digital fluorescence imaging system. We will synchronize our cells, post hoc, based on the time of mitosis; this will allow to determine the time course of how transporter activities change at and near mitosis, which has never before been attempted. The proposed work would lead to the most comprehensive description of pH(i) regulation, and its control by mitogens, in any cell. Moreover, combining the experimental work with the modeling will provide new insights into the factors important for pH(i) regulation. Extending our understanding of pH(i) regulation in MCs both under control conditions and after stimulation by mitogens, could improve our insight into the pathogenesis of glomerular disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Program Projects (P01)
Project #
5P01DK017433-25
Application #
6270422
Study Section
Project Start
1997-12-01
Project End
1998-11-30
Budget Start
1997-10-01
Budget End
1998-09-30
Support Year
25
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
Yale University
Department
Type
DUNS #
082359691
City
New Haven
State
CT
Country
United States
Zip Code
06520

  Publications

Kim, Jun-Mo; Xu, Shuhua; Guo, Xiaoyun et al. (2018) Urinary bladder hypertrophy characteristic of male ROMK Bartter's mice does not occur in female mice. Am J Physiol Regul Integr Comp Physiol 314:R334-R341
Gassaway, Brandon M; Petersen, Max C; Surovtseva, Yulia V et al. (2018) PKC? contributes to lipid-induced insulin resistance through cross talk with p70S6K and through previously unknown regulators of insulin signaling. Proc Natl Acad Sci U S A 115:E8996-E9005
Gilder, Allison L; Chapin, Hannah C; Padovano, Valeria et al. (2018) Newly synthesized polycystin-1 takes different trafficking pathways to the apical and ciliary membranes. Traffic 19:933-945
Barber, Karl W; Muir, Paul; Szeligowski, Richard V et al. (2018) Encoding human serine phosphopeptides in bacteria for proteome-wide identification of phosphorylation-dependent interactions. Nat Biotechnol 36:638-644
Scholl, Ute I; Stölting, Gabriel; Schewe, Julia et al. (2018) CLCN2 chloride channel mutations in familial hyperaldosteronism type II. Nat Genet 50:349-354
Barber, Karl W; Rinehart, Jesse (2018) The ABCs of PTMs. Nat Chem Biol 14:188-192
Barber, Karl W; Miller, Chad J; Jun, Jay W et al. (2018) Kinase Substrate Profiling Using a Proteome-wide Serine-Oriented Human Peptide Library. Biochemistry 57:4717-4725
Castañeda-Bueno, Maria; Arroyo, Juan Pablo; Zhang, Junhui et al. (2017) Phosphorylation by PKC and PKA regulate the kinase activity and downstream signaling of WNK4. Proc Natl Acad Sci U S A 114:E879-E886
Mohler, Kyle; Aerni, Hans-Rudolf; Gassaway, Brandon et al. (2017) MS-READ: Quantitative measurement of amino acid incorporation. Biochim Biophys Acta Gen Subj 1861:3081-3088
D'Lima, Nadia G; Khitun, Alexandra; Rosenbloom, Aaron D et al. (2017) Comparative Proteomics Enables Identification of Nonannotated Cold Shock Proteins in E. coli. J Proteome Res 16:3722-3731

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