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Short food deprivation inhibits orexin receptor 1 expression and orexin-A induced intracellular calcium signaling in acutely isolated duodenal enterocytes

Bengtsson, Magnus W. (författare)
Uppsala universitet,Institutionen för neurovetenskap
Mäkelä, Kari (författare)
Oulu University, Finland
Herzig, Karl-Heinz (författare)
Oulu University, Finland
visa fler...
Flemström, Gunnar (författare)
Uppsala universitet,Institutionen för neurovetenskap
visa färre...
 (creator_code:org_t)
American Physiological Society, 2009
2009
Engelska.
Ingår i: American Journal of Physiology - Gastrointestinal and Liver Physiology. - : American Physiological Society. - 0193-1857 .- 1522-1547. ; 296:3, s. G651-G658
  • Tidskriftsartikel (refereegranskat)
Abstract Ämnesord
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  • Bengtsson MW, Makela K, Herzig KH, Flemstrom G. Short food deprivation   inhibits orexin receptor 1 expression and orexin-A induced   intracellular calcium signaling in acutely isolated duodenal   enterocytes. Am J Physiol Gastrointest Liver Physiol 296: G651-G658,   2009. First published December 31, 2008;   doi:10.1152/ajpgi.90387.2008.-Close intra-arterial infusion of the   appetite regulating peptide orexin-A stimulates bicarbonate secretion   from the duodenal mucosa. The aim of the present study was to elucidate   the ability of orexin-A to induce intracellular calcium signaling in   acutely isolated duodenal enterocytes. Freshly isolated clusters of   enterocytes, obtained from rat duodenal mucosa or human duodenal   biopsies, were loaded with fura 2-AM and mounted in a perfusion   chamber. Cryptlike enterocytes were selected (caged), and changes in   intracellular calcium concentration ([Ca2+](i)) were evaluated by   fluorescence imaging. Total RNA was extracted from pellets of   enterocytes and reverse transcribed to cDNA, and expression of orexin   receptors 1 and 2 (OX1R and OX2R) was measured by quantitative   real-time PCR. Orexin-A at all concentrations tested (1-100 nM)   increased [Ca2+](i) in enterocytes isolated from continuously fed rats,   and the OX1R-antagonist SB-334867 (10 nM) attenuated the response. The   primary [Ca2+](i) response was a slow increase to a sustained plateau   persisting after orexin-A removal, and a similar response was observed   in enterocytes from human biopsies. In contrast to orexin-A, the OX2R   agonist (Ala(11), D-Leu(15))orexin-B (1-10 nM) did not induce calcium   signaling. There were no significant [Ca2+](i) responses in enterocytes   from animals food deprived overnight, and overnight fasting decreased   (P < 0.01) enterocyte OX1R as well as OX2R mRNA. Induction of   intracellular calcium signaling in isolated duodenal enterocytes is   thus mediated primarily by OX1R receptors. Short (overnight) food   deprivation markedly depresses receptor expression and inhibits   orexin-A induced increases in [Ca2+](i). Studies of enterocyte   signaling and intestinal secretion requires particular evaluation   regarding feeding status.

Nyckelord

(Ala(11)
D-Leu(15))-orexin-B
bicarbonate secretion
fasting
feeding
SB-334867
MEDICINE
MEDICIN

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