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我国地带性土壤中产蛋白酶细菌生态分布研究 总被引:2,自引:0,他引:2
按我国土壤地理地带分布,从北到南采土样32个,从中分得细菌491株,并对每一菌株进行了形态学观察与描述。用透明圈法半定量测定各菌株产蛋白酶的活力。对其中产酶活性较高的菌株进行了摇瓶液体培养,定量测定了产蛋白酶的活力。根据细菌分布的数量与活性,分析了生态条件与产酶细菌分布的规律,得出了一些有意义的结果。 相似文献
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细胞凋亡(Apoptosis)与癌基因 总被引:10,自引:0,他引:10
细胞凋亡是细胞衰老、死亡过程的主要形式.最近研究发现有多种癌基因与抑癌基因参与细胞凋亡过程.因此目前认为癌基因与抑癌基因不仅控制细胞增殖、分化,而且调节细胞凋亡.细胞凋亡受阻或缺陷可能是肿瘤发生的基础之一. 相似文献
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A gene (lipP, 837 bp in length) coding for a cold-adapted lipase of psychrophilic bacterium Moritella sp. 2-5-10-1 isolated from Antarctic region was cloned and sequenced in this study. The deduced amino acid sequence revealed
a protein of 278 amino acid residues with a molecular mass of 30,521. The primary structure of the lipase deduced from the
nucleotide sequence showed consensus pentapeptide containing the active serine [Gly-Trp-Ser-Leu-Gly] and a conserved His-Gly
dipeptide in the N-terminal part of the enzyme. These sequences were involved in the lipase active site conformation. Structure
factors that would allow proper enzyme flexibility at low temperatures were discussed. It was suggested that the changes in
the primary structure of the psychrophilic lipases compared to the thermophilic ones could account for their ability to catalyze
lipolysis at temperatures close to 0°C. For expression, the sequence corresponding to the cold-adapted lipase of strain 2-5-10-1
was subcloned into the pET-28a expression vector to construct a recombinant lipase protein. Expression of the lipase by Escherichia coli BL21 (DE3) cells was observed as clear halos on 1% (vol/vol) tributyrin upon induction with IPTG at 25°C. 相似文献
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Mammalian LGN/AGS3 proteins and their Drosophila Pins orthologue are cytoplasmic regulators of G-protein signaling. In Drosophila, Pins localizes to the lateral cortex of polarized epithelial cells and to the apical cortex of neuroblasts where it plays important roles in their asymmetric division. Using overexpression studies in different cell line systems, we demonstrate here that, like Drosophila Pins, LGN can exhibit enriched localization at the cell cortex, depending on the cell cycle and the culture system used. We find that in WISH, PC12, and NRK but not COS cells, LGN is largely directed to the cell cortex during mitosis. Overexpression of truncated protein domains further identified the Galpha-binding C-terminal portion of LGN as a sufficient domain for cortical localization in cell culture. In mitotic COS cells that normally do not exhibit cortical LGN localization, LGN is redirected to the cell cortex upon overexpression of Galpha subunits of heterotrimeric G-proteins. The results also show that the cortical localization of LGN is dependent on microfilaments and that interfering with LGN function in cultured cell lines causes early disruption to cell cycle progression. 相似文献
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Syntaxin-1A binds the nucleotide-binding folds of sulphonylurea receptor 1 to regulate the KATP channel 总被引:3,自引:0,他引:3
Pasyk EA Kang Y Huang X Cui N Sheu L Gaisano HY 《The Journal of biological chemistry》2004,279(6):4234-4240
ATP-sensitive potassium (KATP) channels in neuron and neuroendocrine cells consist of a pore-forming Kir6.2 and regulatory sulfonylurea receptor (SUR1) subunits, which are regulated by ATP and ADP. SNARE protein syntaxin 1A (Syn-1A) is known to mediate exocytic fusion, and more recently, to also bind and modulate membrane-repolarizing voltage-gated K+ channels. Here we show that Syn-1A acts as an endogenous regulator of KATP channels capable of closing these channels when cytosolic ATP concentrations were lowered. Botulinum neurotoxin C1 cleavage of endogenous Syn-1A in insulinoma HIT-T15 cells resulted in the increase in KATP currents, which could be subsequently inhibited by recombinant Syn-1A. Whereas Syn-1A binds both nucleotide-binding folds (NBF-1 and NBF-2) of SUR1, the functional inhibition of KATP channels in rat islet beta-cells by Syn-1A seems to be mediated primarily by its interactions with NBF-1. These inhibitory actions of Syn-1A can be reversed by physiologic concentrations of ADP and by diazoxide. Syn-1A therefore acts to fine-tune the regulation of KATP channels during dynamic changes in cytosolic ATP and ADP concentrations. These actions of Syn-1A on KATP channels contribute to the role of Syn-1A in coordinating the sequence of ionic and exocytic events leading to secretion. 相似文献
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Wenhui Zhang Yuqing Chen Xiaohang Pei Yuzhu Zang Shuangyin Han 《Saudi Journal of Biological Sciences》2018,25(2):242-247
Objective
To investigate the role of DR4 gene in the occurrence, development and prognosis of acute myeloid leukemia (AML), find a new regulatory gene of Decitabine for the treatment of AML, namely DR4 gene, and explore the molecular mechanism of AML in the treatment of AML.Methods
The methylation level and the mRNA expression level of DR4 gene promoters of bone marrow mononuclear cells in 122 patients with newly diagnosed AML and 24 patients with iron deficiency anemia (IDA) were detected using Methylation specific PCR (MS-PCR) and Q-RT-PCR, respectively, and a correlation analysis of them was conducted. The effects of Decitabine on the proliferation of K562 cells were detected using CCK-8 assay. Then, the effects of Decitabine on the methylation level and the mRNA expression level of DR4 genes of K562 cells treated with Decitabine were detected using MS-PCR and Q-RT-PCR, respectively. The effects of Decitabine on the cell cycle and apoptosis of K562 cells were detected using flow cytometry.Results
Compared with the control group, the methylation level (P?=?.002) of DR4 genes of bone marrow mononuclear cells in patients with newly diagnosed AML was high. The methylation level (P?=?.01) of DR4 genes of bone marrow mononuclear cells in patients of the positive group of enlargement of liver, spleen and lymph node was lower than that of the negative group, and the methylation level (P?=?.006) of DR4 genes in patients of the high risk group of clinical stage was lower than that of the low risk group, and the methylation level (P?=?.03) of DR4 genes in patients of the group where patients did not achieve complete remission (CR1) after a course of induction chemotherapy was lower than that of the group where patients achieved complete remission (CR1) after a course of induction chemotherapy. There was a significant negative correlation (P?<?.01) between the methylation level and the mRNA expression level of DR4 genes of bone marrow mononuclear cells in 122 patients with newly diagnosed AML. After the K562 cells were treated with Decitabine for 48?h, the methylation level of DR4 gene promoters gradually decreased, while the mRNA expression level of DR4 genes gradually increased, both of which showed a concentration-dependent relationship. After the K562 cells were treated with 5?µmol/L Decitabine for 48?h, the K562 cells in G0/G1 phase and G2/M phase increased significantly, and the K562 cells in S phase decreased significantly.Conclusion
DR4 gene played an important role in the occurrence and development of AML. Decitabine can effectively inhibit the proliferation of K562 cells, which probably partly because it can terminate the methylation effect of DR4 gene promoters and restore the mRNA expression of DR4 genes. 相似文献109.
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