以淀粉珠为载体的亲和层析法分离纯化高温α淀粉酶

 以淀粉珠为载体的亲和层析法分离纯化高温α淀粉酶张学忠,宋伦,王群,吴晓霞,唐锌进（吉林大学酶工程国家重点实验室,长春１３００２３;南京师范大学生物系,南京２１００２４）金凤燮等人从酒曲中筛选出高产热稳定α淀粉酶的菌株,命名为Ｂａｃｉｌｌｕｓｓｐ－ＪＦ...     

The circular RNA circSlc7a11 promotes bone cancer pain pathogenesis in rats by modulating LLC-WRC 256 cell proliferation and apoptosis

Molecular and Cellular Biochemistry - Treatment of bone cancer pain (BCP) caused by bone metastasis in advanced cancers remains a challenge in clinical oncology, and the underlying mechanisms of...     

蓝光对保护地蔬菜烟粉虱的控制作用

[目的]研究蓝光开灯时段、蓝光光强对烟粉虱Bemisia tabaci (Gennadius)的驱避作用,以及蓝光照射对保护地辣椒和黄瓜上烟粉虱的控制作用,为利用驱虫灯实施对蔬菜烟粉虱的绿色防控提供科学依据.[方法]在蔬菜上用蓝光(波长为470 nm)照射,设置照射时间段17:00-18:00、18:00-19:00、19:00-20:00、20:00-21:00和21:00-22:005个处理、光照强度1、2、6、8、10、20、30、70、1501x9个处理,分别研究不同开灯时段和光强对烟粉虱的驱避作用,以不用蓝光处理为对照;分别在保护地黄瓜和辣椒上放置蓝色灯带,每天18:00-20:00开灯,每3d一次,分别调查黄瓜和辣椒上烟粉虱的虫量.[结果]18:00-19:00时间段蓝光照射对蔬菜烟粉虱的驱避作用最强,虫口减退率占试验总时段的50.94％;17:00-18:00次之,占22.29％;烟粉虱的虫口减退率与光照强度呈正相关(P＜0.05),其回归方程为)y=3.0297x+ 12.508 (R2=0.981).蓝光对保护地辣椒和黄瓜上烟粉虱有较好的驱避作用,辣椒上蓝光处理10d后烟粉虱的虫口减退率达到85.73％,上部叶片和中部叶片上虫口减退率之间没有显著差异(P＞0.05);蓝光处理黄瓜12d后烟粉虱的虫口减退率达90.33％,在光照的前期上部叶片的虫口减退率高于中部叶片,处理9d后上部叶片和中部叶片上虫口减退率之间没有显著差异(P＞0.05).[结论]蓝光对蔬菜烟粉虱具有较强的驱避作用,在18:00-19:00使用蓝光对保护地蔬菜上的烟粉虱的控制效果较好.     

蓝藻Hox氢酶催化产氢的调控

蓝藻是唯一能通过光合作用产生清洁可再生燃料氢气的原核微生物。一些蓝藻具有催化产氢活性的镍-铁Hox氢酶(双向氢酶), 由于其巨大的应用潜力受到广泛的关注。但Hox氢酶在蓝藻产氢过程中调控途径尚不清楚。本文对蓝藻Hox氢酶的结构、生态分布和表达调控的研究进展进行了总结。简单介绍了作者近来对模式蓝藻Synechocystis sp. PCC 6803 hox操纵子中两个未知功能基因ssl2420和sll1225的研究结果。     

A novel ultrasensitive bioluminescent receptor-binding assay of INSL3 through chemical conjugation with nanoluciferase

Insulin-like peptide 3 (INSL3) is a reproduction-related peptide hormone belonging to the insulin/relaxin superfamily, which mediates testicular descent in the male fetus, suppresses male germ cell apoptosis and promotes oocyte maturation in adults by activating the relaxin family peptide receptor 2 (RXFP2). To establish an ultrasensitive receptor-binding assay for INSL3−RXFP2 interaction studies, in the present work we labeled a recombinant INSL3 peptide with a newly developed nanoluciferase (NanoLuc) reporter through a convenient chemical conjugation approach, including the introduction of an active disulfide bond to INSL3 by chemical modification and engineering of a 6× His-Cys-NanoLuc carrying a unique exposed cysteine at the N-terminus. The bioluminescent NanoLuc-conjugated INSL3 retained high binding affinity with the target receptor RXFP2 (K_d = 2.0 ± 0.1 nM, n = 3) and was able to sensitively monitor the receptor-binding of a variety of ligands, representing a novel ultrasensitive tracer for non-radioactive receptor-binding assays. Our present chemical conjugation approach could readily be adapted for conjugation of NanoLuc with other proteins, even other macrobiomolecules, for various highly sensitive bioluminescent assays.     

Ectopic Expression of Arabidopsis Glycosyltransferase UGT85A5 Enhances Salt Stress Tolerance in Tobacco

Abiotic stresses greatly influence plant growth and productivity. While glycosyltransferases are widely distributed in plant kingdom, their biological roles in response to abiotic stresses are largely unknown. In this study, a novel Arabidopsis glycosyltransferase gene UGT85A5 was identified as significantly induced by salt stress. Ectopic expression of UGT85A5 in tobacco enhanced the salt stress tolerance in the transgenic plants. There were higher seed germination rates, better plant growth and less chlorophyll loss in transgenic lines compared to wild type plants under salt stress. This enhanced tolerance of salt stress was correlated with increased accumulations of proline and soluble sugars, but with decreases in malondialdehyde accumulation and Na⁺/K⁺ ratio in UGT85A5-expressing tobacco. Furthermore, during salt stress, expression of several carbohydrate metabolism-related genes including those for sucrose synthase, sucrose-phosphate synthase, hexose transporter and a group2 LEA protein were obviously upregulated in UGT85A5-expressing transgenic plants compared with wild type controls. Thus, these findings suggest a specific protective role of this glycosyltransferase against salt stress and provide a genetic engineering strategy to improve salt tolerance of crops.     

EA15, MIR22, LINC00472 as diagnostic markers for diabetic kidney disease

This study aimed to investigate the molecular mechanisms of diabetic kidney disease (DKD) and to explore new potential therapeutic strategies and biomarkers for DKD. First we analyzed the differentially expressed changes between patients with DKD and the control group using the chip data in Gene Expression Omnibus (GEO) database. Then the gene chip was subjected to be annotated again, so as to screen long noncoding RNAs (lncRNAs) and study expression differences of these lncRNAs in DKD and controlled samples. At last, the function of the differential lncRNAs was analyzed. A total of 252 lncRNAs were identified, and 14 were differentially expressed. In addition, there were 1,629 differentially expressed messenger RNAs (mRNAs) genes, and proliferation and apoptosis adapter protein 15 (PEA15), MIR22, and long intergenic nonprotein coding RNA 472 ( LINC00472) were significantly differentially expressed in DKD samples. Through functional analysis of the encoding genes coexpressed by the three lncRNAs, we found these genes were mainly enriched in type 1 diabetes and autoimmune thyroid disease pathways, whereas in Gene Ontology (GO) function classification, they were also mainly enriched in the immune response, type I interferon signaling pathways, interferon-γ mediated signaling pathways, and so forth. To summary, we identified EA15, MIR22, and LINC00472 may serve as the potential diagnostic markers of DKD.     

CKIP-1 regulates the immunomodulatory function of mesenchymal stem cells

Molecular Biology Reports - Mesenchymal stem cells (MSCs) are self-renewing multipotent cells with immunoregulatory function, which makes them attractive candidates for regenerative medicine....     

Expression of a modified Cry1Ie gene in E. coli and in transgenic tobacco confers resistance to corn borer

The wild-type Crylle gene from Bacillus thuringiensis was modified for its efficient expression in transgenic plants. Modified Crylle gene (designated as Cryllem) was cloned into prokaryotic expressionvector pET28b and its expression in E.coli was confirmed by SDS-PAGE analysis. Bioassays using crude expression products in E.coli revealed that CrylIem protein had a similar toxicity to corn borer as wild-type CrylIe. CrylIem gene was then inserted downstream of the maize ubiquitin-1 promoter in plant expression vector p3301. Transgenic tobacco plants carrying Cryllem showed insecticidal activity against corn borer.