Literature DB >> 1191698

Energy-dependent calcium uptake activity of microsomes from the aorta of normal and hypertensive rats.

L Moore, L Hurwitz, G R Davenport, E J Landon.   

Abstract

Energy-dependent calcium uptake activity of microsomes isolated from the rat aorta has been characterized. The microsomes consist of smooth membrane vesicles which in the presence of MG-ATP as an energy source continuously sequester calcium over a 60-min period. This calcium uptake is greatly stimulated by oxalate anion which serves as a calcium trapping agent. Unlike the calcium uptake of mitochondria this uptake is not inhibited by sodium azide. Sucrose density gradient analysis of the microsomal calcium uptake suggests that the system is associated with the sarcoplasmic reticulum. In presence of 5 mM Mg-ATP and 20 muM calcium approximately 38 nmol of calcium per mg of microsomal protein are taken up in 20 min. In the absence of ATP, less than 2 nmol of calcium per mg of protein are taken up in the first 2 min with no further uptake of calcium in subsequent time periods. When calcium uptake activity is plotted against calcium or ATP concentration of the medium, half maximal activity is calculated for 24.3 muM calcium and for 1.6 mM ATP. The calcium uptake characteristics of the rat aorta microsomes are compatible with a postulated role in the relaxation of the vascular smooth muscle and the provision of an intracellular calcium store for muscle contraction. Aorta microsomes from SHR rats (a genetic strain that is spontaneously hypertensive) have a significantly reduced uptake when compared with the corresponding nonhypertensive control strain. The level of calcium and ATP for half maximal activity of the rat aorta microsomal calcium uptake system is approximately the same in the SHR and the control strain. The rate of release of calcium from rat aorta microsomes is apparently identical in SHR strain and control. The calcium uptake activity of kidney and liver microsomes isolated from the SHR strain and control. The calcium uptake activity of kidney and liver microsomes isolated from the SHR rat appears to be identical to that found in the control strain.

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Year:  1975        PMID: 1191698     DOI: 10.1016/0005-2736(75)90126-1

Source DB:  PubMed          Journal:  Biochim Biophys Acta        ISSN: 0006-3002


  11 in total

1.  Evidence for a visceral smooth muscle abnormality in Okamoto spontaneous hypertension.

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3.  Properties of energy-dependent calcium transport by rat liver microsomal fraction as revealed by initial-rate measurements.

Authors:  F L Bygrave
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4.  Electron cytochemistry of oxalate-stimulated calcium uptake in microsomes from the smooth muscle of the pig stomach.

Authors:  L Raeymaekers; B Agostini; W Hasselbach
Journal:  Histochemistry       Date:  1980-02

5.  Blood pressure development of the spontaneously hypertensive rat after concurrent manipulations of dietary Ca2+ and Na+. Relation to intestinal Ca2+ fluxes.

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6.  Vascular reactivity in hypertension: altered effect of ouabain.

Authors:  R C Webb; D F Bohr
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7.  Reactivity to bradykinin and potassium of the isolated duodenum from rats with genetic and renal hypertension.

Authors:  N Miasiro; T B Paiva; C C Pereira; S I Shimuta
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8.  Calcium leakage as a cause of the high resting tension in vascular smooth muscle from the spontaneously hypertensive rat.

Authors:  J P Noon; P J Rice; R J Baldessarini
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Review 9.  Symphony of vascular contraction: how smooth muscle cells lose harmony to signal increased vascular resistance in hypertension.

Authors:  Styliani Goulopoulou; R Clinton Webb
Journal:  Hypertension       Date:  2014-01-27       Impact factor: 10.190

10.  Decreased content of integral membrane calcium-binding protein (IMCAL) in tissues of the spontaneously hypertensive rat.

Authors:  S Kowarski; L A Cowen; D Schachter
Journal:  Proc Natl Acad Sci U S A       Date:  1986-02       Impact factor: 11.205

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