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951.
A simple assay procedure for carmine and carminic acid samples 总被引:2,自引:0,他引:2
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Nocardia species aromatized 19-hydroxyprogesterone, 3beta, 19-dihydroxy-pregn-5-en-20-one 3-acetate and pregn-5-ene-3beta, 19, 20beta-triol 3-acetate, without cleavage of the side chain, into 3-hydroxy-19-norpregna-1,3,5 (10)-trien-20-one. Septomyxa affinis aromatized the ring A and cleaved the side chain of 19-hydroxyprogesterone to yield estrone. With 19-hydroxypregna-4, 7-diene-3, 20-dione as substrate, the transformation was more complex and many products were formed. 相似文献
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The plaque organs of Pyrops consist of elaborately folded, finely perforated cuticular areas, each associated with numerous bipolar sensory cells organised in groups. The proximal, mitochondrial region of each dendrite narrows to reveal a ciliary ultrastructure. The ciliary fibrils pass into a highly vesiculated region and beyond this are succeeded by a dense array of neurotubules. Peripherally the dendrites proliferate numerous fine branches from which finer filaments extend into the cuticular pores. The plaques are considered to be complex olfactory organs evolved from groups of sensilla basiconica. 相似文献
958.
An enzymically catalysed reaction between d-glucose and the protein cyst coat of the ciliate Colpoda steinii 总被引:2,自引:2,他引:0
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1. The isolated protein cyst coat of Colpoda steinii reacted with [(14)C]glucose to bind (14)C label in a reaction that was not an artifact of bacterial contamination or of adsorption. 2. The reaction was enzymically catalysed, had optimum pH7.0-7.4 and a temperature optimum of 36-38 degrees C, was non-competitively and reversibly inhibited by 10mum-p-hydroxymercuribenzoate and was specific for d-glucose. It had K(m)8.2x10(-6)m. 3. With the exception of C-1, all the carbon atoms of glucose were bound to the same extent and, measured relative to C-2 or C-6, the binding of C-1 varied between 0.45 and 0.82. The lost C-1 was not accounted for as carbon dioxide. 4. On prolonged incubation a coat preparation reacted with 3.6% of its own weight of glucose. 5. The label was tightly bound, but after acid treatment a variable proportion was recovered as glucose and there was no evidence for the release of any other (14)C-containing compound. 6. Even after dissolution of the coat protein, bound label was not removed by treatment with periodate or lead tetra-acetate. 相似文献
959.
Ribosomal Ribonucleic Acid-Adenine (N6-) Methylase of Escherichia coli Strain B: Ionic and Substrate Site Requirements
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These investigations are concerned with the ionic and substrate-site requirements of ribosomal ribonucleic acid (rRNA)-adenine (N(6)-) methylase of Escherichia coli B. The methylase was essentially inactive in solutions of low ionic strength. The addition of MgCl(2) (optimal at 5 mM) or; to a lesser degree, KCl (optimal at 45 mM) stimulated the rate of methylation; the combination of MgCl(2) and KCl stimulated methylation to an extent equivalent to the sum of the stimulation of each acting alone. The extent of nonspecific binding of the methylase to rRNA decreased as the ionic strength of the solution increased. In the absence of ions, dimethylsulfoxide (DMSO), a nucleic acid denaturing agent, had little influence on the rate of methylation; however, DMSO plus KCl synergistically increased both the rate and the extent of methylation to a greater degree than the combination of Mg(2+) plus K(+). NH(4) (+) was less effective than K(+), and the divalent Mg(2+) offered little stimulation. Monovalent anions (acetate, nitrate, and chloride) were equally effective, whereas divalent SO(4) (2-) was decidedly inhibitory. The appropriate ionic milieu of mono- and divalent cations was required to provide the appropriate conformation of the rRNA and to facilitate specific interactions of the methylase and its recognition sites in the rRNA, while decreasing nonspecific ionic binding of the methylase to rRNA. DMSO may facilitate methylation by increasing the number of substrate sites exposed in single-stranded regions of the rRNA. Nonmethylatable rRNA species served as competitive inhibitors, whereas the polyanions deoxyribonucleic acid, transfer RNA, and polyadenylic acid were inactive. Micrococcus lysodeikticus and Bacillus subtilis rRNA, methylated by the methylase, each contained two distinct heptanucleotides containing newly synthesized 6-methyladenine moieties. The data are consistent with the view that E. coli strain B possesses two species of rRNA-adenine (N(6)-) methylases, each of which recognizes a specific adenine moiety in a unique pentapurine nucleotide sequence in a single-stranded region of rRNA. 相似文献
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