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Pattern formation mechanisms in developing organisms determine cellular differentiation and function. However, the components that interact during the manifestation of a spatial pattern are in general unknown. Characean algae represent a model system to study pattern formation. These algae develop alternating acid and alkaline transport domains that influence the pattern of growth. In the present study, it will be demonstrated that a diffusion mechanism is implicated in acid and alkaline domain formation and this growth pattern. Experiments on the characean growth pattern were performed that resulted in pronounced, however, unpredictable modifications in the original pattern. A major component involved in this pattern-forming mechanism emerged from the nonlinear kinetics of the H+-ATPase that is located in the plasma membrane of these algae. Based on these kinetics, a mathematical model was developed and numerically analyzed. As a result, the contribution of a diffusional component to the characean acid/alkaline pattern appeared most likely.This work was supported by the Deutsche Forschungsgemeinschaft (grant #571 1/1) to JF.  相似文献   
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Using the cDNA of bovine lung prostaglandin F synthase (EC 1.1.1.2) as a probe, we isolated a clone from a bovine liver cDNA library which differed in only eleven nucleotides from the probe. The corresponding protein contained three amino acid substitutions, including a leucine residue which is conserved throughout all aldo-keto reductases. We inserted the liver cDNA into expression vector pUC19 and expressed the recombinant liver enzyme in E.coli. The purified liver enzyme reduced prostaglandin H2 as well as prostaglandin D2 and various carbonyl compounds. The high relative activity against prostaglandin H2 in combination with a high Km value for prostaglandin D2 identified this liver enzyme as a lung type prostaglandin F synthase. However, the binding constant for NADPH of the liver enzyme was 3.5 fold higher than that of lung prostaglandin F synthase.  相似文献   
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Cells of the white blood series infiltrate ovarian follicles during the ovulatory process. A segment of the wall of periovulatory ovine follicles was incubated and conditioned media subjected to ultrafiltration. Leukocyte chemoattractant activity of media was measured using a linear under-agarose migration assay. Bioactivity was recovered following filtration through a 3000 molecular weight cut-off membrane. Filtrate was then fractionated by reverse phase high performance liquid chromatography. Peptides recovered from two fractions with significant chemoattractant activity were sequenced. One fraction contained 16 amino acid residues with repeating triplets of Gly-X-Y, where X and Y were often proline and hydroxyproline, respectively. Because this motif is characteristic of alpha collagens, and since thecal collagen is degraded during the mechanics of ovulation, it appears that this chemoattractant is derived from the connective tissue matrix of the follicle. Peptide isolated from the other bioactive chromatographic fraction was 15 amino acids in length, and rich in glycine, but did not contain imino acids. To our knowledge this is the first report of purification of leukocyte chemoattractants of reproductive tissue origin. Resident follicular granulocytes and mononuclear cells are capable of secreting a broad spectrum of potent chemicals that could be involved in the mechanisms of ovulation and luteinization.  相似文献   
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To study the effects of exercise intensity and duration on excess postexercise oxygen consumption (EPOC), 8 men [age = 27.6 (SD 3.8) years, VO2max = 46.1 (SD 8.5) ml min-1 kg-1] performed four randomly assigned cycle-ergometer tests (20 min at 60% VO2max, 40 min at 60% VO2max, 20 min at 70% VO2max, and 40 min at 70% VO2max). O2 uptake, heart rate and rectal temperature were measured before, during, and for 1 h following the exercise tests. Blood for plasma lactate measurements was obtained via cannulae before, and at selected times, during and following exercise. VO2 rapidly declined to preexercise levels following each of the four testing sessions, and there were no differences in EPOC between the sessions. Blood lactate and rectal temperature increased (P < 0.05) with exercise, but had returned to preexercise levels by 40 min of recovery. The results indicate that VO2 returned to resting levels within 40 min after the end of exercise, regardless of the intensity (60% and 70% VO2max) or duration (20 min and 40 min) of the exercise, in men with a moderate aerobic fitness level.  相似文献   
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