Abstract

The main objective is to examine the cellular and molecular mechanisms responsible for the regulation of acid-base transport by the renal cortical collecting duct (CCD). Studies performed in our laboratory have shown that there are at least two functionally different types of intercalated cells in the CCD of mature rabbits: one secretes H+ via a luminal H+ATPase (type A) and one secretes HCO3 via an apical Cl/HCO3 exchanger (type B). Type A cells show rapid apical endocytotic activity, whereas type B cells bind peanut agglutinin (PNA). These properties facilitate their identification by functional fluorescent dyes. Exposure to acidic media results in alteration of intercalated cell physiology, characterized by the loss of apical Cl/HCO3 exchangers by some type B cells and conversion of net HCO3 transport by CCDs from secretion to absorption. Although type A cells can be stimulated to increase H+ secretion in response to acid treatment, the cellular mechanisms underlying the response are not well understood; little is known how the type B cells respond. We have suggested that they might be able to reverse functional polarity and secrete H+, but alternative explanations are possible, To address this polarity issue directly we plan to perfuse CCDs at low pH in vitro, using a fluorescent pH sensitive dye (BCECF) to estimate fluxes of H+/HCO3 in individual intercalated cells before and after the incubation. The molecular mechanisms underlying changes in physiology of both subtypes of intercalated cells will be examined by determining the duration of the acid stimulus needed to set off these changes, as well as any requirement for protein synthesis, signal transduction or microfilament-microtubular function. Functional changes will be correlated with fluorescent immunocytochemical studies using antibodies to specific apical and basolateral Cl/HCO3 exchangers, and H+ATPases, as well as Western blots and 2-D protein gels of acid-incubated CCDs. To determine when intercalated cells become competent to transport H+/HCO3 and respond to acid loading, CCDs from mesonephric, neonatal, and maturing kidneys will be incubated in acidic media and examined as described above. Isolated CCDs, as well as a subconfluent (""""""""immature"""""""") collecting duct cell line, will be examined by in situ hybridization for the disappearance of proliferative and pattern-formation genes and appearance of acid-base related (differentiated) genes. Finally, since developing intercalated cells might not express mature phenotypes, their lineage will be determined in the neonatal rat kidney using retrovirus-mediated gene transfer. The results of these studies should help us to better understand at the cellular level how the intercalated cell develops and differentiates and how the kidney responds to metabolic acidosis. They also should help to explain why the newborn is less able to regulate acid-base homeostasis than is the adult.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Eunice Kennedy Shriver National Institute of Child Health & Human Development (NICHD)
Type
Research Project (R01)
Project #
5R01HD013232-13
Application #
3312135
Study Section
General Medicine B Study Section (GMB)
Project Start
1990-07-01
Project End
1995-02-28
Budget Start
1991-03-01
Budget End
1992-02-29
Support Year
13
Fiscal Year
1991
Total Cost
Indirect Cost

  Institution

Name
Albert Einstein College of Medicine
Department
Type
Schools of Medicine
DUNS #
009095365
City
Bronx
State
NY
Country
United States
Zip Code
10461

  Publications

Matsumoto, T; Fejes-Toth, G; Schwartz, G J (1996) Postnatal differentiation of rabbit collecting duct intercalated cells. Pediatr Res 39:1-12
Brion, L P; Zavilowitz, B J; Suarez, C et al. (1994) Metabolic acidosis stimulates carbonic anhydrase activity in rabbit proximal tubule and medullary collecting duct. Am J Physiol 266:F185-95
Schwartz, G J; Brown, D; Mankus, R et al. (1994) Low pH enhances expression of carbonic anhydrase II by cultured rat inner medullary collecting duct cells. Am J Physiol 266:C508-14
Satlin, L M; Yasoshima, K; Schwartz, G J (1994) H+ secretion in rabbit mesonephric collecting tubule. Am J Physiol 267:F979-86
Matsumoto, T; Winkler, C A; Brion, L P et al. (1994) Expression of acid-base-related proteins in mesonephric kidney of the rabbit. Am J Physiol 267:F987-97
Schwartz, G J; Winkler, C A; Zavilowitz, B J et al. (1993) Carbonic anhydrase II mRNA is induced in rabbit kidney cortex during chronic metabolic acidosis. Am J Physiol 265:F764-72
Matsumoto, T; Fejes-Toth, G; Schweartz, G J (1993) Developmental expression of acid-base-related proteins in the rabbit kidney. Pediatr Nephrol 7:792-7
Schwartz, G J; Zavilowitz, B J; Radice, A D et al. (1992) Maturation of aldose reductase expression in the neonatal rat inner medulla. J Clin Invest 90:1275-83
Schwartz, G J (1992) Does kL/PCr estimate GFR, or does GFR determine k? Pediatr Nephrol 6:512-5
Yasoshima, K; Satlin, L M; Schwartz, G J (1992) Adaptation of rabbit cortical collecting duct to in vitro acid incubation. Am J Physiol 263:F749-56

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