Controlling and Defence‐related Mechanisms of Bacillus Strains Against Bacterial Leaf Blight of Rice

Bacillus strains are broadly studied for their beneficial role in plant growth and biological control of plant disease and pest; however, little is known about their underlying mechanisms. In this study, we assessed the controlling and defence‐related mechanisms of three Bacillus strains including rice seed‐associated strain B. subtilis A15, rhizobacterial strains B. amyloliquefaciens D29 and B. methylotrophicus H8, all of which are against bacterial leaf blight (BLB) caused by Xanthomonas oryzae pv. oryzae. Results indicated that all three strains showed strong biofilm formation ability. The culture filtrates of each strain significantly suppressed the growth and biofilm formation of X. oryzae, while changes in bacterial cell morphology such as cell swell and severe cell wall alterations were observed through the transmission electron microscopy images. PCR analysis revealed that all three strains harbour the antimicrobial‐associated genes that are responsible for biosynthesis of bacillomycin, fengycin, iturin and surfactin. Subsequent real‐time qPCR analysis revealed the upregulated expression of fenD and srfAA genes in D29 and H8, and fenD and ituC genes in A15 during their in vitro interaction with X. oryzae. It suggests that the antibacterial mechanisms of the three strains may be at least partially associated with their ability to secrete corresponding lipopeptides. Interestingly, the applications of the three strains in greenhouse conditions were found to be effective in controlling the BLB disease, which was achieved through the activation of inducing systemic resistance resulted from the enhanced activities of defence‐related enzymes. This is the first report of demonstration of the mode of antibacterial effect of Bacillus strains against X. oryzae. Overall, data from the current study provide valuable information for biological control of BLB disease in rice.     

Palmitic acid induces human osteoblast-like Saos-2 cell apoptosis via endoplasmic reticulum stress and autophagy

Palmitic acid (PA) is the most common saturated long-chain fatty acid in food that causes cell apoptosis. However, little is known about the molecular mechanisms of PA toxicity. In this study, we explore the effects of PA on proliferation and apoptosis in human osteoblast-like Saos-2 cells and uncover the signaling pathways involved in the process. Our study showed that endoplasmic reticulum (ER) stress and autophagy are involved in PA-induced Saos-2 cell apoptosis. We found that PA inhibited the viability of Saos-2 cells in a dose- and time-dependent manner. At the same time, PA induced the expression of ER stress marker genes (glucose-regulated protein 78 (GRP78) and CCAAT/enhancer binding protein homologous protein (CHOP)), altered autophagy-related gene expression (microtubule-associated protein 1 light chain 3 (LC3), ATG5, p62, and Beclin), promoted apoptosis-related gene expression (Caspase 3 and BAX), and affected autophagic flux. Inhibiting ER stress with 4-PBA diminished the PA-induced cell apoptosis, activated autophagy, and increased the expression of Caspase 3 and BAX. Inhibiting autophagy with 3-MA attenuated the PA and ER stress-induced cell apoptosis and the apoptosis-related gene expression (Caspase 3 and BAX), but seemed to have no obvious effects on ER stress, although the CHOP expression was downregulated. Taken together, our results suggest that PA-induced Saos-2 cell apoptosis is activated via ER stress and autophagy, and the activation of autophagy depends on the ER stress during this process.     

Role of c-fos gene in vasoactive intestinal peptide promoted synthesis of pulmonary surfactant phospholipids

We previously reported that vasoactive intestinal peptide (VIP) promoted synthesis of phosphatidylcholine (PC) in alveolar type II (ATII) cells. But the intracellular mechanism for this effect was unknown. In this work, we investigated the intracellular signal transduction pathway for VIP promoted synthesis of PC, the major lipid component of pulmonary surfactant (PS), by using an antagonist of VIP receptors, inhibitor of protein kinase C (PKC) and antisense oligonucleotides (AS-ODN) for c-fos oncogene. Our results showed that: ① [D-P-Cl-Phe(6)-Leu(17)]-VIP (10^− 6 mol/l), an antagonist of VIP receptors, could decrease the quantity of [³H] choline incorporation, microsomal choline-phosphate cytidylyltransferase (CCT) mRNA expression and CCT activity induced by VIP (10^− 8 mol/l) in cultured lung explants to the control levels; ② VIP (10^− 8 mol/l) upregulated c-Fos protein expression in ATII cells. AS-ODN for c-fos oncogene (9 × 10^− 6 mol/l) could block the elevation of [³H] choline incorporation, microsomal CCT mRNA expression and CCT activity induced by VIP in cultured lung explants and in ATII cells; ③ H7 (10^− 5 mol/l), a PKC inhibitor could also reduce VIP induced [³H] choline incorporation, microsomal CCT mRNA expression and CCT activity in cultured lung explants and in ATII cells. These results demonstrated that VIP receptors, PKC and c-Fos protein played important roles in the signaling pathway through which VIP promoted the synthesis of PC.     

内含子数量改变GUS基因的瞬时表达调控

内含子是基因的重要组成部分,它与功能基因表达之间的关系越来越被重视.本研究以pCAMBIA3301为载体,利用玉米泛素启动子Ubi1和水稻肌动蛋白启动子Actin1构建两个GUS基因表达载体p33U1和p33A1,同时设置3个对照载体.通过基因枪轰击法将上述载体转入水稻胚性愈伤组织,探讨内含子对外源目的基因表达的调控作用.组织化学检测结果表明:CaMV35S启动子调控下的iGUS (带内含子)基因能够顺利表达;同样,Actin1启动子(带内含子)调控下的不带内含子的GUS基因也可以正常表达,而当Actin1启动子(带内含子)驱动iGUS基因时,则导致GUS染色反应不能发生.Ubi1启动子(带内含子)调控GUS基因的瞬时表达也得出类似结果,证明表达框中内含子的数量为1个或两个时,对GUS基因的表达起到了不同的调控作用.本研究结果对植物表达载体构建及功能基因表达都具有指导意义.     

板蓝根水提物S-03体外抑制甲、乙型流感病毒感染的实验研究

以水提法分离制备板蓝根水提物S-03分析其基本化学成分,并在狗肾细胞(MDCK)上分别接种人甲1、3型和乙型流感病毒标准株、临床分离株以及禽流感病毒,采用空斑减少和免疫荧光及血凝抑制实验方法,在预防、治疗和直接作用三种试验模式下探讨S-03体外对流感病毒的抑制作用。研究结果表明S-03的主要化学成分为糖类,多糖所占总重的比例最高。S-03体外抗病毒药效显示:①预防模式:对各型流感病毒均无抑制作用;②治疗和直接作用模式:对不同亚型流感病毒均有一定程度的抑制作用,且直接作用(SI=2.5~16)效果优于治疗模式(SI=2.2~5.8);③血凝抑制试验:对不同亚型的人流感病毒血凝素有不同程度抑制作用(最低抑制浓度为3.12~25 mg/mL),并且对禽流感病毒(H6N2、H7N3、H9N2)的血凝素也有一定的抑制作用(最低抑制浓度25~50 mg/mL),其作用机制可能为抑制流感病毒表面的血凝素(HA),从而阻止病毒感染。     

Structure and protective effect of exopolysaccharide from P. Agglomerans strain KFS-9 against UV radiation

The water-soluble exopolysaccharide (WSEPS) from Pantoea agglomerans strain KFS-9 isolated from mangrove forest was prepared by removing bacterial cell from the fermentation liquid following by concentration and cold ethanol precipitation of the supernatant. The polysaccharide material was purified by gel permeation chromatography on a Sephacryl S-300HR column and characterized using chemical and spectral methods. The results show that WSEPS is protein-bound polysaccharide, and it is composed of arabinose, glucose galactose and gulcuronic acid in the molar ratio of 1.0:2.2:2.8:0.9. Their antioxidant activities in vitro were studied by various antioxidant assays, including hydroxyl radical scavenging, superoxide radical scavenging and antilipid peroxidation. The results show that the WSEPS extracted had a high antioxidant activity in a concentration-dependent manner (except the activity of antilipid peroxidation). WSEPS quenched hydroxyl radicals, superoxide radicals at low amounts, the IC(50) of which were 0.07 and 0.15 mg/ml, respectively. These results indicate that the protective effect of WSEPS against UV radiation is most likely to be due to the free radicals-scavenging ability.     

Eukaryotic proteins expressed in Escherichia coli: an improved thrombin cleavage and purification procedure of fusion proteins with glutathione S-transferase

Several systems have been developed to allow for rapid and efficient purification of recombinant proteins expressed in bacteria. The expression of polypeptides in frame with glutathione S-transferase (GST) allows for purification of the fusion proteins from crude bacterial extracts under nondenaturing conditions by affinity chromatography on glutathione agarose (D. B. Smith and K. S. Johnson, 1988, Gene 67, 31-40). This vector expression system has also incorporated specific protease cleavage sites to facilitate proteolysis of the bacterial fusion proteins. In our hands, the cleavage of these fusion proteins at a thrombin cleavage site proceeded slowly. To facilitate the cleavage of fusion proteins, we have introduced a glycine-rich linker (glycine kinker) containing the sequence P.G.I.S.G.G.G.G.G located immediately following the thrombin cleavage site. This glycine kinker greatly increases the thrombin cleavage efficiency of several fusion proteins. The introduction of the glycine kinker into fusion proteins allows for the cleavage of the fusion proteins while they are attached to the affinity resin resulting in a single step purification of the recombinant protein. More than 2 mg of the highly purified protein was obtained from the equivalent of 100 ml of bacterial culture within a few hours when a protein tyrosine phosphatase was employed as a test protein. The vector, pGEX-KG, has also been modified to facilitate cloning of a variety of cDNAs in all reading frames and has been successfully used to express several eukaryotic proteins.