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SYNOPSIS. A symbiotic alga from the foraminifer Archaias angulatus was isolated axenically. Algae from crushed hosts were coccoid and highly vacuolated; division stages within an envelope were common. Biflagellate motile piriform organisms predominated in newly transferred cultures and were gradually replaced by the coccoid, highly vacuolated stage. Incorporation of 14C label in intact Archaias was greatest for organisms fed and incubated in light. Starved symbiotized organisms incubated in the light incorporated ~30% as much label as fed counterparts, There was no obvious difference in 45Ca incorporation between fed and starved organisms. Light significantly enhanced calcification. The Archaias symbiont infected Rosalina leei but not Quinqueloculina spp. 相似文献
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A third vitamin B12 binding protein present in normal serum has been shown to participate in transport of labelled vitamin B12 absorbed from the gut. All three vitamin B12 binding proteins in serum were labelled at the same time after oral administration of vitamin B12, implying that “free” vitamin B12 reached the portal blood from the gut mucosa. 相似文献
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Dependence of Betaine Stimulation of Vitamin B12 Overproduction on Protein Synthesis 总被引:1,自引:0,他引:1 下载免费PDF全文
The betaine-stimulated differential synthesis of vitamin B12, i.e., the increase in B12 per increase in dry cell weight, by Pseudomonas denitrificans was inhibited by rifampin and chloramphenicol but not by benzylpenicillin and carbenicillin at concentrations of antibiotic that inhibit growth. The level of the first enzyme of corrin (and porphyrin) biosynthesis, δ-aminolevulinic acid synthetase, was decreased to a much greater degree by rifampin and chloramphenicol than by the penicillins. These data support the concept that betaine stimulation of B12 synthesis is a result of its stimulation of synthesis of δ-aminolevulinic acid synthetase, a labile and presumably rate-limiting enzyme of corrin formation requiring continuous induction. In further support of this hypothesis, it was found that chloramphenicol immediately interfered with both vitamin B12 and δ-aminolevulinic acid synthetase formation, no matter when it was added to the system. 相似文献
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DONALD L. WISE 《The Journal of eukaryotic microbiology》1968,15(3):528-531
SYNOPSIS. Eight mM acetaldehyde prevented growth of Polytomella caeca in acetate medium and differentially changed the labeling by acetate-2-14C of chromatographically separated RNA hydrolysate products. Four mM acetaldehyde also prevented growth in acetate medium unless uridine, thymidine, guanosine, uracil, thymine or quanine were present; then growth was delayed by 2 or 4 days. Orotidine, orotic acid, dihydroortic acid, cytosine, cytidine, adenosine and adenine had no effect on growth in acetate medium containing 4 mM acetaldehyde. One mM acetaldehyde promoted growth in acetate medium and also could serve as a sole carbon source. One mM propionaldehyde, but not butyraldehyde, was also an adequate carbon source. Four mM acetaldehyde, as a sole carbon source, supported growth only when uridine was present. 相似文献
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The protein bCblC (bCblCpro) is a bovine homolog of a human B12 trafficking chaperone that is responsible for the processing of vitamin B12 and its escorted delivery in intracellular B12 metabolism. In this study, we found that bCblCpro is highly thermolabile with a T
m = 42.0 ± 0.2 °C as shown for the human homolog, suggesting thermal regulation of these proteins. Binding of the reduced form
of glutathione (GSH) that is a predominant cellular thiol increased the T
m of bCblCpro from 42 °C to ~45 °C (ΔT
m max = 3.1 ± 0.2 °C and AC50 = 2.1 ± 0.5 mM). Binding of vitamin B12 and its derivatives also stabilized bCblCpro increasing the T
m to a different extent and vitamin B12 (cyanocobalamin, CNCbl) was the least efficient (ΔT
m max = 4.3 ± 0.3 °C and AC50 = 291 ± 36 μM). However, the stabilizing effect of CNCbl was significantly greater for GSH-bound bCblCpro (ΔT
m max = 12.8 ± 0.6 °C and AC50 = 9.3 ± 1.6 μM) than for GSH-free bCblCpro. In addition, the stabilizing effect of GSH was also greater for CNCbl-bound bCblCpro
(ΔT
m max = 9.3 ± 0.3 °C and AC50 = 57.0 ± 6.8 μM). Limited proteolysis revealed that thermal stabilization of bCblCpro is derived from conformational changes
of the protein induced by binding of the ligands. The results in this study indicate that GSH cooperates with vitamin B12 in thermal stabilization of bCblCpro and is a positive regulator of the protein. 相似文献
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Various species of Micromonospora produced yields of vitamin B(12) activity as high as 11 mug/ml under conditions of shaken flask fermentation. 相似文献
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D. Sean Froese Jolanta Kopec Fiona Fitzpatrick Marion Schuller Thomas J. McCorvie Rod Chalk Tanja Plessl Victoria Fettelschoss Brian Fowler Matthias R. Baumgartner Wyatt W. Yue 《The Journal of biological chemistry》2015,290(49):29167-29177
Conversion of vitamin B12 (cobalamin, Cbl) into the cofactor forms methyl-Cbl (MeCbl) and adenosyl-Cbl (AdoCbl) is required for the function of two crucial enzymes, mitochondrial methylmalonyl-CoA mutase and cytosolic methionine synthase, respectively. The intracellular proteins MMACHC and MMADHC play important roles in processing and targeting the Cbl cofactor to its destination enzymes, and recent evidence suggests that they may interact while performing these essential trafficking functions. To better understand the molecular basis of this interaction, we have mapped the crucial protein regions required, indicate that Cbl is likely processed by MMACHC prior to interaction with MMADHC, and identify patient mutations on both proteins that interfere with complex formation, via different mechanisms. We further report the crystal structure of the MMADHC C-terminal region at 2.2 Å resolution, revealing a modified nitroreductase fold with surprising homology to MMACHC despite their poor sequence conservation. Because MMADHC demonstrates no known enzymatic activity, we propose it as the first protein known to repurpose the nitroreductase fold solely for protein-protein interaction. Using small angle x-ray scattering, we reveal the MMACHC-MMADHC complex as a 1:1 heterodimer and provide a structural model of this interaction, where the interaction region overlaps with the MMACHC-Cbl binding site. Together, our findings provide novel structural evidence and mechanistic insight into an essential biological process, whereby an intracellular “trafficking chaperone” highly specific for a trace element cofactor functions via protein-protein interaction, which is disrupted by inherited disease mutations. 相似文献
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In Euglena gracilis, vitamin B12 uptake follows a biphasic patternconsisting of an initial rapid phase followed by a slower secondaryphase. Chase experiments showed that vitamin B12 was tightlybound to its receptor-sites during either rapid or slow phaseof uptake. The slow phase was markedly inhibited when Euglenacells were preincubated with cycloheximide for 30 min at a concentrationof 100µg/ml. When the preincubation time was longer than30 min, a gradual inhibition of the rapid phase occurred andreached 84% after 4 h. This inhibitory effect of cycloheximideis reversible. On the other hand, tunicamycin at 1 µ/mlirreversibly inhibited the B12 uptake suggesting that the receptor-sitefor B12 is glycoprotein in nature. These results suggest thatthe rapid phase is also dependent on protein synthesis and representsB12 binding on preexisting free receptors whereas the secondaryslow phase represents Bl2 binding on newly synthesized receptors.Both phases of uptake seem to be controled by the same receptor.The half-life of the free receptor is estimated to be 66 minwhereas the B12 receptor complex is very stable. (Received October 3, 1988; Accepted February 15, 1989) 相似文献
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ESTELA NOVAK EDNA FREYMULLER HAAPALAINEN SOLANGE DA SILVA JOSE FRANCO DA SILVEIRA 《The Journal of eukaryotic microbiology》1988,35(3):375-378
Here we describe a method that allows the isolation of intact trypanosomatid symbionts in amounts sufficient for biochemical analysis. The isolated symbionts retain their characteristic morphological features and are reasonably free of subcellular debris. They actively incorporate [3H]leucine and [35S]methionine into proteins. Chloramphenicol and rifampicin at 50 μg/ml almost completely inhibit the incorporation of protein precursors. The inhibition of protein synthesis by the antibiotics provides direct evidence for the existence of a prokaryotic protein-synthesizing system in this unusual intracellular structure. The pattern of protein synthesis of the isolated symbionts is complex. Several symbiont polypeptides are absent or poorly represented in the flagellate. 相似文献
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《Journal of Fermentation and Bioengineering》1993,75(3):182-186
We isolated about 500 isopropanol(IPA)-assimilating bacteria from many soil samples, among which 23 strains produced vitamin B12. Taxonomical studies of the best producer, designated strain Hi16.3, showed that it belonged to the genus Arthrobacter. Vitamin B12 production by the strain was higher than that by 12 other authentic Arthrobacter spp. using glucose as a sole carbon source. In fed-batch culture, the maximum production yield with strain Hi16.3 (named A. hyalinus) was 2 mg/l in the culture broth, when 80 ml of IPA/l broth was consumed. 相似文献
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Vitamin B(12) production by a newly isolated strain of a methanol-utilizing bacterium was studied. The maximal yield of the vitamin, 2.6 mg/liter of medium was attained by optimization. 相似文献
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S. G. Jeffs 《BMJ (Clinical research ed.)》1960,2(5200):732-733
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C. C. Ungley 《BMJ (Clinical research ed.)》1949,2(4641):1370-1377