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Iris Seed Dormancy 总被引:1,自引:0,他引:1
Iris embryos were treated in several ways to study the cause of delayed germination. The results of this work indicate that a chemical inhibitor is present in the endosperm and mechanical inhibition of embryo growth also occurs. The mechanical inhibition reduces excised Iris embryo growth to the same extent as does the chemical inhibitor. 相似文献
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A method for the activation and measurement of insect prophenol oxidase using nitrocellulose membrane is presented. Using this method we were able to conveniently activate both crude and purified prophenol oxidase from insects belonging to three different orders. This rapid method allows for prophenol oxidase activation, in the absence of a prophenol oxidase-activating system, and in the presence of high ionic strength, protease inhibitors, or chelator. 相似文献
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Demonstration of the presence of an ultrafiltrable substance in human serum activating somatomedin A
M H Heulin M Artur J Straczek D Malaprade M Pierson J F Stoltz F Belleville P Paysant P Nabet 《Comptes rendus des séances de la Société de biologie et de ses filiales》1981,175(3):364-371
Human serum contains an ultrafiltrable factor which stimulates the somatomedin activity measured by 35SO4 incorporation into pelvic cartilage of chick embryo, this ultrafiltrable factor activates native serum somatomedin or partially purified somatomedin. The molecular weight determined by fractionated ultrafiltration or chromatography on Biogel P2 is about 350-500 daltons. 相似文献
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Alejandro A. Pezzulo Patrick H. Kelly Boulos S. Nassar Cedric J. Rutland Nicholas D. Gansemer Cassie L. Dohrn Andrew J. Costello David A. Stoltz Joseph Zabner 《Applied and environmental microbiology》2013,79(19):5936-5941
Human lungs are constantly exposed to bacteria in the environment, yet the prevailing dogma is that healthy lungs are sterile. DNA sequencing-based studies of pulmonary bacterial diversity challenge this notion. However, DNA-based microbial analysis currently fails to distinguish between DNA from live bacteria and that from bacteria that have been killed by lung immune mechanisms, potentially causing overestimation of bacterial abundance and diversity. We investigated whether bacterial DNA recovered from lungs represents live or dead bacteria in bronchoalveolar lavage (BAL) fluid and lung samples in young healthy pigs. Live bacterial DNA was DNase I resistant and became DNase I sensitive upon human antimicrobial-mediated killing in vitro. We determined live and total bacterial DNA loads in porcine BAL fluid and lung tissue by comparing DNase I-treated versus untreated samples. In contrast to the case for BAL fluid, we were unable to culture bacteria from most lung homogenates. Surprisingly, total bacterial DNA was abundant in both BAL fluid and lung homogenates. In BAL fluid, 63% was DNase I sensitive. In 6 out of 11 lung homogenates, all bacterial DNA was DNase I sensitive, suggesting a predominance of dead bacteria; in the remaining homogenates, 94% was DNase I sensitive, and bacterial diversity determined by 16S rRNA gene sequencing was similar in DNase I-treated and untreated samples. Healthy pig lungs are mostly sterile yet contain abundant DNase I-sensitive DNA from inhaled and aspirated bacteria killed by pulmonary host defense mechanisms. This approach and conceptual framework will improve analysis of the lung microbiome in disease. 相似文献