The in-situ oxidation of manganese sulfate solution with H2O_(2),sodium hypochlorite,potassium permanganate and oxygen as oxidants was investigated by means of SEM,EDS,XRD,BET and infrared analysis,and the effects of ...The in-situ oxidation of manganese sulfate solution with H2O_(2),sodium hypochlorite,potassium permanganate and oxygen as oxidants was investigated by means of SEM,EDS,XRD,BET and infrared analysis,and the effects of different oxidants on the morphology,phase composition,surface properties and specific surface area of manganese oxides were investigated.The experimental results show that the diameter of manganese oxide particles prepared with H_(2)O_(2)is the smallest,about 50 nm,and the specific surface area is the largest,63.8764 m^(2)/g.It has the advantages of abundant surface hydroxyl groups,no introduction of other impurities and large adsorption potential.It is most suitable to be used as an oxidant for oxidizing manganese sulfate solution to prepare manganese oxide by in-situ oxidation.Nano manganese oxide prepard by H_(2)O_(2)in-situ oxidation method is used as adsorbent to adsorb cobalt and nickel impurities in manganese sulfate.When the reaction pH is 6,the reaction time is 30min and the amount of adsorbent is 1.0 g,the adsorption rates of cobalt and nickel impurities in 100ml manganese sulfate solution are 97.59%and 97.67%,respectively.The residual amounts of cobalt and nickel meet the industrial process standard of first-class products(Co,Ni w/%≤0.005)of high-purity manganese sulfate(Hg/t4823-2015)for batteries.The study plays a guiding role in the preparation and regulation of manganese oxide,and provides a new method with high efficiency,purity and adsorbent availability for the preparation of high-purity manganese sulfate solution.展开更多
目的通过NHE1基因敲除模型鼠的海马组织差异蛋白质组学分析,发现并明确Ppp3cb和Ppm1g的表达特征。方法①选取6只2周龄NHE1基因敲除模型鼠作为模型组,同周龄野生型小鼠6只作为对照组,采用琼脂糖凝胶电泳检测其基因型;应用旷场实验和强迫...目的通过NHE1基因敲除模型鼠的海马组织差异蛋白质组学分析,发现并明确Ppp3cb和Ppm1g的表达特征。方法①选取6只2周龄NHE1基因敲除模型鼠作为模型组,同周龄野生型小鼠6只作为对照组,采用琼脂糖凝胶电泳检测其基因型;应用旷场实验和强迫游泳实验对模型组和对照组小鼠进行行为学评估,并按照Racine评分标准对模型鼠进行癫痫发作分级;②通过串联质谱分析技术对模型组和对照组的海马组织进行差异蛋白筛选,基因本体论(Gene Ontology Analysis,GO)分析差异蛋白并进行注释和富集,蛋白网络数据库(search tool for the retrieval of interesting genes,STRING)分析差异蛋白之间的蛋白相互作用(protein-protein interaction,PPI);③应用qPCR和Western blot检测Ppp3cb和Ppm1g的转录和翻译水平,应用免疫组织化学技术分别观察其在组织中的表达量。结果①模型组小鼠NHE1基因未见表达,旷场实验中模型鼠的运动总距离较对照组减少(P=0.0073),跨越的格子数比对照组显著减少(P<0.0001)。强迫游泳实验结果显示,模型鼠不动的时间明显延长(P<0.0001);②以表达倍数(FC)≥1.2倍且P<0.05为筛选标准,检测到海马组织中845个差异表达的蛋白质点,其中有9个蛋白表达上调,7个蛋白表达下调。其中Ppp3cb下调,Ppm1g上调。GO功能注释结果表明,NHE1敲除后,分子功能(MF)富集在蛋白丝氨酸/苏氨酸磷酸酶活性的差异最显著,细胞成分(CC)富集在质膜部分的差异蛋白数量最多,生物过程(BP)富集在负向调节生物过程、免疫系统过程的差异蛋白数量最多。STRING分析显示差异蛋白Ppp3cb和Slc9a1直接作用,Ppm1g通过Ppp3cb和Slc9a1间接作用,Ppp3cb和Ppm1g之间相互作用。③Ppp3cb的转录和翻译水平减少,在组织中的表达量下降,而Ppm1g转录和翻译水平增加,在组织中的表达量上升(P<0.05)。结论本研究确定了NHE1基因敲除小鼠海马组织中差异蛋白Ppp3cb表达下调,而Ppm1g表达上调,为进一步研究Ppp3cb和Ppm1g参与癫痫发病机制提供了依据。展开更多
背景:骨关节炎是一种常见的由关节软骨退行性改变所导致的关节慢性炎症,越来越多的研究表明机械应力与骨关节炎的发展密切相关。Hippo通路既参与机体组织细胞发育又是机械应力的效应因子,参与调控骨代谢和软骨代谢。目的:通过调控Hippo...背景:骨关节炎是一种常见的由关节软骨退行性改变所导致的关节慢性炎症,越来越多的研究表明机械应力与骨关节炎的发展密切相关。Hippo通路既参与机体组织细胞发育又是机械应力的效应因子,参与调控骨代谢和软骨代谢。目的:通过调控Hippo通路可能成为干预骨关节炎的新靶点之一,因而此文通过对机械应力调控Hippo通路影响骨关节炎的研究进行综述,以期为骨关节炎的发病机制提供思路并对骨关节炎的治疗方法提供新的理论依据。方法:采用PubMed、Web of Science、Embase、中国知网、维普及万方数据库进行文献检索,检索各数据库建库至2023年有关机械应力对骨关节炎的影响及机械应力、Hippo通路与骨关节炎相关的所有文献,最终纳入75篇文献进行综述。结果与结论:①不同机械应力对骨关节炎的细胞增殖凋亡与分化、骨关节炎症与血管稳态发挥不同的作用;②坚硬细胞外基质、低细胞密度、中等剪切力、中等拉伸力及压缩力通过活化YAP/TAZ可达到细胞增殖、成骨分化、血管稳态及抑制炎症反应的作用;③软细胞外基质、高细胞密度、过度剪切力、过度拉伸力及压缩力通过失活YAP/TAZ进而抑制细胞增殖、促软骨分化、破坏血管稳态及促进炎症反应,促进骨关节炎进程。展开更多
基金Funded by the National Natural Science Foundation of China(No.51864012)the Key Projects Supported by Science and Technology in Guizhou Province(No.[2002]KEY020)+2 种基金the Major Special Projects in Guizhou Province(No.[2022]003)the Guizhou Provincial Science Cooperation Program(Nos.[2016]5302,[2017]5788,[2018]5781,[2019]1411,and[2019]2841)the Major Special Projects in Tongren City,Guizhou Province(No.[2021]13)。
文摘The in-situ oxidation of manganese sulfate solution with H2O_(2),sodium hypochlorite,potassium permanganate and oxygen as oxidants was investigated by means of SEM,EDS,XRD,BET and infrared analysis,and the effects of different oxidants on the morphology,phase composition,surface properties and specific surface area of manganese oxides were investigated.The experimental results show that the diameter of manganese oxide particles prepared with H_(2)O_(2)is the smallest,about 50 nm,and the specific surface area is the largest,63.8764 m^(2)/g.It has the advantages of abundant surface hydroxyl groups,no introduction of other impurities and large adsorption potential.It is most suitable to be used as an oxidant for oxidizing manganese sulfate solution to prepare manganese oxide by in-situ oxidation.Nano manganese oxide prepard by H_(2)O_(2)in-situ oxidation method is used as adsorbent to adsorb cobalt and nickel impurities in manganese sulfate.When the reaction pH is 6,the reaction time is 30min and the amount of adsorbent is 1.0 g,the adsorption rates of cobalt and nickel impurities in 100ml manganese sulfate solution are 97.59%and 97.67%,respectively.The residual amounts of cobalt and nickel meet the industrial process standard of first-class products(Co,Ni w/%≤0.005)of high-purity manganese sulfate(Hg/t4823-2015)for batteries.The study plays a guiding role in the preparation and regulation of manganese oxide,and provides a new method with high efficiency,purity and adsorbent availability for the preparation of high-purity manganese sulfate solution.
文摘目的通过NHE1基因敲除模型鼠的海马组织差异蛋白质组学分析,发现并明确Ppp3cb和Ppm1g的表达特征。方法①选取6只2周龄NHE1基因敲除模型鼠作为模型组,同周龄野生型小鼠6只作为对照组,采用琼脂糖凝胶电泳检测其基因型;应用旷场实验和强迫游泳实验对模型组和对照组小鼠进行行为学评估,并按照Racine评分标准对模型鼠进行癫痫发作分级;②通过串联质谱分析技术对模型组和对照组的海马组织进行差异蛋白筛选,基因本体论(Gene Ontology Analysis,GO)分析差异蛋白并进行注释和富集,蛋白网络数据库(search tool for the retrieval of interesting genes,STRING)分析差异蛋白之间的蛋白相互作用(protein-protein interaction,PPI);③应用qPCR和Western blot检测Ppp3cb和Ppm1g的转录和翻译水平,应用免疫组织化学技术分别观察其在组织中的表达量。结果①模型组小鼠NHE1基因未见表达,旷场实验中模型鼠的运动总距离较对照组减少(P=0.0073),跨越的格子数比对照组显著减少(P<0.0001)。强迫游泳实验结果显示,模型鼠不动的时间明显延长(P<0.0001);②以表达倍数(FC)≥1.2倍且P<0.05为筛选标准,检测到海马组织中845个差异表达的蛋白质点,其中有9个蛋白表达上调,7个蛋白表达下调。其中Ppp3cb下调,Ppm1g上调。GO功能注释结果表明,NHE1敲除后,分子功能(MF)富集在蛋白丝氨酸/苏氨酸磷酸酶活性的差异最显著,细胞成分(CC)富集在质膜部分的差异蛋白数量最多,生物过程(BP)富集在负向调节生物过程、免疫系统过程的差异蛋白数量最多。STRING分析显示差异蛋白Ppp3cb和Slc9a1直接作用,Ppm1g通过Ppp3cb和Slc9a1间接作用,Ppp3cb和Ppm1g之间相互作用。③Ppp3cb的转录和翻译水平减少,在组织中的表达量下降,而Ppm1g转录和翻译水平增加,在组织中的表达量上升(P<0.05)。结论本研究确定了NHE1基因敲除小鼠海马组织中差异蛋白Ppp3cb表达下调,而Ppm1g表达上调,为进一步研究Ppp3cb和Ppm1g参与癫痫发病机制提供了依据。
文摘背景:骨关节炎是一种常见的由关节软骨退行性改变所导致的关节慢性炎症,越来越多的研究表明机械应力与骨关节炎的发展密切相关。Hippo通路既参与机体组织细胞发育又是机械应力的效应因子,参与调控骨代谢和软骨代谢。目的:通过调控Hippo通路可能成为干预骨关节炎的新靶点之一,因而此文通过对机械应力调控Hippo通路影响骨关节炎的研究进行综述,以期为骨关节炎的发病机制提供思路并对骨关节炎的治疗方法提供新的理论依据。方法:采用PubMed、Web of Science、Embase、中国知网、维普及万方数据库进行文献检索,检索各数据库建库至2023年有关机械应力对骨关节炎的影响及机械应力、Hippo通路与骨关节炎相关的所有文献,最终纳入75篇文献进行综述。结果与结论:①不同机械应力对骨关节炎的细胞增殖凋亡与分化、骨关节炎症与血管稳态发挥不同的作用;②坚硬细胞外基质、低细胞密度、中等剪切力、中等拉伸力及压缩力通过活化YAP/TAZ可达到细胞增殖、成骨分化、血管稳态及抑制炎症反应的作用;③软细胞外基质、高细胞密度、过度剪切力、过度拉伸力及压缩力通过失活YAP/TAZ进而抑制细胞增殖、促软骨分化、破坏血管稳态及促进炎症反应,促进骨关节炎进程。