Abstract

Over the past 5 years, we have focused on studies aiming at understanding the response and adaptation of brainstem neurons to O2 deprivation. Our results have indicated that the response of brainstem neurons to hypoxia is different from that of cortical neurons. During hypoxia, brainstem neurons depolarize and increase their excitability to raise motoneuronal output, while excitability of cortical neurons decreases. This decrease in neuronal excitability may delay injury in cortical neurons, but it is not clear how brainstem neurons protect themselves from excessive depolarization and hypoxic damage. In this regard, our preliminary data have shown that activation of ATP-sensitive K+ (Katp) channels occurs during hypoxia and this may attenuate the hypoxia-induced depolarization and limit the increased neuronal excitability. We believe that this is an important finding as its implications are not limited only to brainstem neurons, but also applied to all neurons that are endowed with these channels. In spite of this, Katp channel regulation in central neurons is not well understood, especially during hypoxia. In order to determine the role of these Katp channels during O2 deprivation and their regulation by a number of cytosolic and membrane factors, we have developed this experimental proposal. Three major hypotheses will be tested: 1) hypoxia activates Katp channels in brainstem neurons and this improves the functional recovery of these neurons post hypoxia; 2) activation of Katp channels during hypoxia is a result of interactive changes in several cytosolic and membrane factors; and 3) Katp channel activity is modulated by endogenous neurotransmitters in a G protein-dependent manner. Several techniques will be used including single channel recordings in excised and cell-attached patches, whole-cell voltage clamp in acutely dissociated neurons, measurements of ionic concentrations with ion-selective microelectrodes and intracellular recordings from brainstem slices. All of these techniques are currently operative in our laboratory. Two groups of neurons (hypoglossal neurons and non-respiratory neurons in the substantia nigra) will be used in these experiments, both of which have a high density of Katp channels. We believe that our proposed studies will yield important new information that will improve our understanding of how these Katp channels are regulated in central neurons at zest and during hypoxia. We wish that this new knowledge will lead to a design of more effective therapeutical strategies in preventing or diminishing hypoxia/ischemia- induced brain injury.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL058410-04
Application #
6056428
Study Section
Respiratory and Applied Physiology Study Section (RAP)
Project Start
1996-09-01
Project End
2001-03-31
Budget Start
1999-09-01
Budget End
2001-03-31
Support Year
4
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Georgia State University
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
837322494
City
Atlanta
State
GA
Country
United States
Zip Code
30302

  Publications

Cui, Ningren; Li, Li; Wang, Xueren et al. (2006) Elimination of allosteric modulation of myocardial KATP channels by ATP and protons in two Kir6.2 polymorphisms found in sudden cardiac death. Physiol Genomics 25:105-15
Su, Junda; Jiang, Chun (2006) Multicellular recordings of cultured brainstem neurons in microelectrode arrays. Cell Tissue Res 326:25-33
Li, Li; Shi, Yun; Wang, Xueren et al. (2005) Single nucleotide polymorphisms in K(ATP) channels: muscular impact on type 2 diabetes. Diabetes 54:1592-7
Wang, R; Rojas, A; Wu, J et al. (2005) Determinant role of membrane helices in K ATP channel gating. J Membr Biol 204:1-10
Wang, Runping; Su, Junda; Wang, Xueren et al. (2005) Subunit stoichiometry of the Kir1.1 channel in proton-dependent gating. J Biol Chem 280:13433-41
Jiang, Chun; Rojas, Asheebo; Wang, Runping et al. (2005) CO2 central chemosensitivity: why are there so many sensing molecules? Respir Physiol Neurobiol 145:115-26
Mao, Jinzhe; Wang, Xueren; Chen, Fuxue et al. (2004) Molecular basis for the inhibition of G protein-coupled inward rectifier K(+) channels by protein kinase C. Proc Natl Acad Sci U S A 101:1087-92
Wu, J; Xu, H; Shen, W et al. (2004) Expression and coexpression of CO2-sensitive Kir channels in brainstem neurons of rats. J Membr Biol 197:179-91
Wu, Jianping; Piao, Hailan; Rojas, Asheebo et al. (2004) Critical protein domains and amino acid residues for gating the KIR6.2 channel by intracellular ATP. J Cell Physiol 198:73-81
Li, Li; Rojas, Asheebo; Wu, Jianping et al. (2004) Disruption of glucose sensing and insulin secretion by ribozyme Kir6.2-gene targeting in insulin-secreting cells. Endocrinology 145:4408-14

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