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11.
Pantoea agglomerans pvs. gypsophilae and betae are related gall-forming bacteria. While P. agglomerans pv. beta initiates gall formation on both beet and gypsophila, the gypsophila pathovar causes gall formation only on gypsophila. PthG is a type III effector determining host range of these pathogens, initiating the hypersensitivity response in beet, but is a virulence factor in gypsophila. The role of PthG and its mode of action in pathogenicity remain unclear. Transgenic Nicotiana tabacum plants expressing pthG were created. PthG over-expression was often lethal, and surviving pthG-bearing lines showed morphological and developmental abnormalities such as leaf deformation and abnormal vascular branching, dwarf stature, loss of apical dominance, seedling apical meristem loss, rapid germination, reduced fertility, plants which cease growth for several weeks later producing a new lateral shoot, and loss of endophyte resistance (bearing unusual saprophyte populations). Some transformants required light for seed germination and showed rapid seedling greening. In in vitro assays PthG expression modified responses to auxin and cytokinin, inhibiting root and shoot production but not callus formation. In vitro differentiation responses to light were modified by PthG expression. This effector may interfere in the plant auxin signalling pathways resulting in higher observed auxin and ethylene levels, and subsequent blockage of root and shoot development. Apparently PthG tunes the host response to high hormone levels, changing the developmental response. Since shoot and root development are delayed, we hypothesize that callus/gall formation is supported by this activity. However, interference by PthG with hormone and light signalling does not explain all the responses observed in pthG-bearing lines.  相似文献   
12.
In apterous adults of the spirea aphid, Aphis citricola van der Goot, the optimum conditions for determining acetylcholinesterase (AChE) activity consist of reaction mixture of 0.1 M phosphate buffer (pH 7.5), 10?3M acetylthiocholine (ASCh), and enzyme extract equivalent to 80 ± 3 μg protein incubated for 15 min at 30°C. The Km value for ASCh (6.7 × 10?5M) was much lower than that of butyrylthiocholine (BuSCh) (1.25 × 10?2M). The enzyme activity was almost completely inhibited by 10?6M paraoxon or 10?5M eserine and was 84% inhibited by 10?5M BW284C51 (a specific AChE inhibitor). DTNB was found to inhibit the enzyme activity and was therefore added at the end of the reaction. AChE activity of A. citricola was inhibited in vitro and in vivo by dimethoxon > dimethoate, and aldicarb sulfoxide > aldicarb > aldicarb sulfone. The in vivo effect correlates well with the toxicity level of the various toxicants. A neurotoxicity index which combines both mortality and in vivo inhibition of the aphid AChE activity is suggested as a measure for determining the toxicity of organophosphorus and carbamate compounds toward aphids.  相似文献   
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