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d-myoInositol 1:2-cyclic phosphate 2-phosphohydrolase   总被引:23,自引:19,他引:4       下载免费PDF全文
1. An enzyme in extracts of mammalian tissues catalyses the hydrolysis of d-myoinositol 1:2-cyclic phosphate (an intermediary in the enzymic degradation of phosphatidylinositol) to produce d-myoinositol 1-phosphate. 2. The enantiomorph of the substrate is not attacked. 3. The pH optimum is about 8.1-8.3 and the reaction is stimulated by Mg(2+) ions. 4. Extracts from rat kidney cortex and medulla are very rich sources of the enzyme; brain, testis and small intestine contain intermediary activities, and other tissues contain very small amounts.  相似文献   

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BOOK REVIEWS: 2     
Karin  Bammann 《Biometrics》2005,61(1):313-314
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BOOK REVIEWS: 2     
VanessaDidelez 《Biometrics》2004,60(4):1057-1057
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BOOK REVIEWS: 2     
S. G. Walker 《Biometrics》2003,59(4):1191-1191
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Workshop 7: 2     
Glutamine, the preferred precursor for neurotransmitter glutamate, is likely to be the principal substrate for the neuronal System A transporter SAT1 in vivo. By measuring currents associated with SAT1 expression in Xenopus oocytes, we found that SAT1 mediates transport of small, neutral, aliphatic amino acids including glutamine, alanine and the System A‐specific analogue 2‐(methylamino) isobutyrate, each with K0.5 of 0.3–0.5 mm . Amino acid transport is driven by the Na+ electrochemical gradient. Kinetic data indicates that Na+/cotransport comprises the ordered binding first of Na+ (a voltage‐dependent step), then alanine, then simultaneous translocation. Li+ (but not H+) can substitute for Na+ but results in reduced Vmax. In the absence of amino acid, SAT1 mediates a cation leak with selectivity Na+, Li+, H+, K+. The temperature‐dependence of the leak current (Ea = 17 ± 3 kcal/mol) is consistent with carrier‐mediated Na+ uniport activity (cf 13 ± 2 kcal/mol for Na+/alanine cotransport) but the leak does not saturate at physiological [Na+], suggesting channel activity. Despite a Na+ Hill coefficient of 1, we obtained Na+/amino acid coupling coefficients greater than 1 from simultaneous measurement of charge and [3H]alanine or [3H]glutamine uptake. Interpretation of these data is model‐dependent and consistent with either (1) an all‐carrier model in which Na+/amino acid cotransport is thermodynamically coupled 2 : 1, cotransport is preferred over Na+ uniport, and in which there is little cooperativity between Na+ binding events, or (2) 1 : 1 coupling in parallel with an always‐on Na+ channel activity. In either scenario, the presence of SAT1 at the plasma membrane and resultant Na+ fluxes will place a significant energy burden on the cell.  相似文献   

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Shock : Part 2     
Paul G. Weil 《CMAJ》1942,46(5):417-423
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BOOK REVIEWS: 2     
G. Heimann 《Biometrics》2003,59(3):736-736
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Book Review: 2     
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Book Reviews: 2     
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BOOK REVIEWS: 2     
Mohammad Fraiwan  Al-Saleh 《Biometrics》2005,61(4):1130-1130
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BOOK REVIEWS: 2     
O. Berke 《Biometrics》2004,60(3):839-840
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