Effects of climate warming on plant autotoxicity in forest evolution: a case simulation analysis for Picea schrenkiana regeneration

In order to explore how plant autotoxicity changes with climate warming, the autotoxicity of P. schrenkiana needles' water extract, organic extract fractions, and key allelochemical DHAP was systemically investigated at the temperature rising 2 and 4°C based on the data‐monitored soil temperature during the last decade in the stage of Schrenk spruce regeneration (seed germination and seedling growth). The results showed that the criterion day and night temperatures were 12°C and 4°C for seed germination, and 14°C and 6°C for seedling growth, respectively. In the presence of water extract, the temperature rise of 2°C significantly inhibited the germination vigor and rate of P. Schrenkiana seed, and a temperature rise of 4°C significantly increased the inhibition to the seedling growth (P < 0.05). Among the three organic fractions, the low‐polar fraction showed to be more phytotoxic than the other two fractions, causing significant inhibitory effects on the seed germination and growth even at low concentration of 0.1 mg/mL, and the inhibition effect was enhanced as temperature increased. The temperature rise significantly enhanced the promotion effect of DHAP, while the inhibition effect of temperature rise became less important with increasing concentration of DHAP. This investigation revealed that autotoxicity of P. schrenkiana was affected by the climate warming. As expected, it provided an insight into the mechanism and effectiveness of allelopathy in bridging the causal relationship between forest evolution and climate warming.     

Improved Tolerance of <Emphasis Type="Italic">Escherichia coli</Emphasis> to Propionic Acid by Overexpression of Sigma Factor RpoS

Propionic acid (PA) is an economically important compound, but large-scale microbial production of PA confronts obstacle such as acid stress on microbial cells. Here, we show that overexpressing sigma factor RpoS improves the acid tolerance of Escherichia coli. Four genes including rpoS, fur, pgi and dnaK (encoding RNA polymerase sigma factor, ferric uptake regulator, phosphoglucoisomerase, and chaperone, respectively) were independently overexpressed in E. coli. The recombinant E. coli overexpressing rpoS showed the highest PA tolerance. This strain could grow in M9 medium at pH 4.62, whereas wild type E. coli survived only at pHs above 5.12. Moreover, in the shake-flask cultivation, the E. coli strain overexpressing rpoS grew faster than wild type. Notably, the minimum inhibitory concentration of PA for this recombinant strain was 7.81 mg/mL, which was 2-fold higher in comparison with wild type. Overall these results indicated that overexpression of sigma factor rpoS significantly enhanced E. coli tolerance to PA.     

A Simple Synthetic Strategy toward Defect‐Rich Porous Monolayer NiFe‐Layered Double Hydroxide Nanosheets for Efficient Electrocatalytic Water Oxidation

In this work, porous monolayer nickel‐iron layered double hydroxide (PM‐LDH) nanosheets with a lateral size of ≈30 nm and a thickness of ≈0.8 nm are successfully synthesized by a facile one‐step strategy. Briefly, an aqueous solution containing Ni²⁺ and Fe³⁺ is added dropwise to an aqueous formamide solution at 80 °C and pH 10, with the PM‐LDH product formed within only 10 min. This fast synthetic strategy introduces an abundance of pores in the monolayer NiFe‐LDH nanosheets, resulting in PM‐LDH containing high concentration of oxygen and cation vacancies, as is confirmed by extended X‐ray absorption fine structure and electron spin resonance measurements. The oxygen and cation vacancies in PM‐LDH act synergistically to increase the electropositivity of the LDH nanosheets, while also enhancing H₂O adsorption and bonding strength of the OH* intermediate formed during water electrooxidation, endowing PM‐LDH with outstanding performance for the oxygen evolution reaction (OER). PM‐LDH offers a very low overpotential (230 mV) for OER at a current density of 10 mA cm^?2, with a Tafel slope of only 47 mV dec^?1, representing one of the best OER performance yet reported for a NiFe‐LDH system. The results encourage the wider utilization of porous monolayer LDH nanosheets in electrocatalysis, catalysis, and solar cells.     

猪源冠状病毒聚合酶基因的克隆及特性分析

参照GenBank中Purdue株序列对TGEV TS株聚合酶基因(ORF1)设计特异性引物,经RT-PCR扩增获得了20054bp的片段,与预期大小相符.TS株与Pur46-MAD株的ORF1核苷酸和氨基酸序列同源性分别为98.8%和99.0%,与FIPV、PEDV、HCV299E及SARS氨基酸同源性分别为88%、57%、57%和45%.不同冠状病毒比较结果显示RdRp有很高的保守性而且有重要的作用,序列分析标明TS株在ORF1a和ORF1b重叠区有核糖体剪切位点UUUAAAC,且相应区域RNA二级结构形成3个茎环结构.     

新型非甾醇蜕皮激素类杀虫剂对棉铃虫幼虫蜕皮的影响

用透射电镜技术研究了新型非甾醇蜕皮激素类杀虫剂W200013对棉铃虫4龄幼虫蜕皮的影响。结果表明W200013使棉铃虫产生早熟、致死的蜕皮。中毒试虫6 h表现出内表皮层沉积加快,皮细胞中粗面型内质网大量增加,糖原颗粒减少;12 h蜕皮间隙开始形成,细胞质凝集;24 h新、旧表皮同时存在,皮细胞空泡化严重;36 h新上表皮覆盖于仅沉积几层的新原表皮上,旧表皮仍然保持,皮细胞呈恶化、降解状态,宏观上虫体不表现出蜕皮行为而死亡。而且比较研究可见W200013在中毒症状、生物测定结果、超微结构水平与RH-5992具有相似的作用。     

Delayed cutaneous wound closure in HO‐2 deficient mice despite normal HO‐1 expression

Impaired wound healing can lead to scarring, and aesthetical and functional problems. The cytoprotective haem oxygenase (HO) enzymes degrade haem into iron, biliverdin and carbon monoxide. HO‐1 deficient mice suffer from chronic inflammatory stress and delayed cutaneous wound healing, while corneal wound healing in HO‐2 deficient mice is impaired with exorbitant inflammation and absence of HO‐1 expression. This study addresses the role of HO‐2 in cutaneous excisional wound healing using HO‐2 knockout (KO) mice. Here, we show that HO‐2 deficiency also delays cutaneous wound closure compared to WT controls. In addition, we detected reduced collagen deposition and vessel density in the wounds of HO‐2 KO mice compared to WT controls. Surprisingly, wound closure in HO‐2 KO mice was accompanied by an inflammatory response comparable to WT mice. HO‐1 induction in HO‐2 deficient skin was also similar to WT controls and may explain this protection against exaggerated cutaneous inflammation but not the delayed wound closure. Proliferation and myofibroblast differentiation were similar in both two genotypes. Next, we screened for candidate genes to explain the observed delayed wound closure, and detected delayed gene and protein expression profiles of the chemokine (C‐X‐C) ligand‐11 (CXCL‐11) in wounds of HO‐2 KO mice. Abnormal regulation of CXCL‐11 has been linked to delayed wound healing and disturbed angiogenesis. However, whether aberrant CXCL‐11 expression in HO‐2 KO mice is caused by or is causing delayed wound healing needs to be further investigated.     

Chemical Constituents of Crinum asiaticum L. var. sinicum Baker and Their Cytotoxic Activities

A phytochemical investigation of the bulbs of Crinum asiaticum L. var. sinicum Baker resulted in the isolation of two new alkaloids, asiaticumines A and B ( 1 and 2 , resp.), together with 21 known compounds, including nine alkaloids, four amides, five phenolic compounds, and three flavonoids. All 23 compounds were isolated for the first time from Crinum asiaticum L. var. sinicum Baker . Their structures were elucidated by spectroscopic methods. In addition, ten alkaloids, 1 – 10 , were evaluated for their cytotoxic activities against human tumor cell lines A549, LOVO, HL‐60, and 6T‐CEM. Compounds 3, 4 , and 7 – 10 selectively showed remarkable inhibition against one or more of the tested cell lines.     

产木聚糖酶白地霉培养特性及部分纯化的酶学特性

本文对白地霉Ref1的培养特性、产酶条件和酶学特性进行了初步研究。结果表明:该菌为低温型菌株,其最佳生长条件为pH6、20℃和酵母膏作为氮源;最佳产酶条件为pH3-7、15℃及以酵母膏氮源;条件优化后产酶可达118.7U/mL,可溶蛋白含量可达到60μg/mL,酶溶液的比活可达到1250U/mg蛋白质;该木聚糖酶的最适反应温度和pH分别为50℃和5,金属离子Mg2+、Na+和8mmol/L的Fe2+、Cu2+、Zn2+等对木聚糖酶的活性有抑制作用,而Ca2+、4mmol/L的Fe2+、Cu2+、Zn2+和8mmol/L的Mn2+等对该酶反应则有促进作用;该木聚糖酶在保温2h后在15-40℃范围内能保持80%以上的酶活性,在50℃时能保持68%的酶活性;用lineweaver-Burk作图法(双倒数作图法)求得该酶的最大反应速度Vmax和Km值分别为163.38mmol/mg/min和0.75mg/mL。     

Soluble uric acid induces myocardial damage through activating the NLRP3 inflammasome

Uric acid crystal is known to activate the NLRP3 inflammasome and to cause tissue damages, which can result in many diseases, such as gout, chronic renal injury and myocardial damage. Meanwhile, soluble uric acid (sUA), before forming crystals, is also related to these diseases. This study was carried out to investigate whether sUA could also activate NLRP3 inflammasome in cardiomyocytes and to analyse the mechanisms. The cardiomyocyte activity was monitored, along with the levels of mature IL‐1β and caspase‐1 from H9c2 cells following sUA stimulus. We found that sUA was able to activate NLRP3 inflammasome, which was responsible for H9c2 cell apoptosis induced by sUA. By elevating TLR6 levels and then activating NF‐κB/p65 signal pathway, sUA promoted NLRP3, pro‐caspase 1 and pro‐IL‐1β production and provided the first signal of NLRP3 inflammasome activation. Meanwhile, ROS production regulated by UCP2 levels also contributed to NLRP3 inflammasome assembly and subsequent caspase 1 activation and mature IL‐1β secretion. In addition, the tlr6 knockdown rats suffering from hyperuricemia showed the lower level of IL‐1β and an ameliorative cardiac function. These findings suggest that sUA activates NLRP3 inflammasome in cardiomyocytes and they may provide one therapeutic strategy for myocardial damage induced by sUA.