The present invention relates to an in-situ miniature lysimeter for intelligent irrigation

本实用新型属于蒸渗仪技术领域，具体涉及一种智能灌溉的原位小型蒸渗仪，包括保护筒、防尘板、土柱桶、钢丝绳、引流器、支座、淋溶液采集器、称重机构、管道、水势传感器、抽水泵、取样器、信号线、控制器、控制线、电子水表、水管，所述保护筒埋设于地面以下，所述保护筒内设置有称重机构，所述称重机构上设置有支座，所述支座上接触有土柱桶，所述土柱桶上设置有引流器。本实用新型将主体装置置于地下环境，能够降低土柱内环境温度、水分等条件与实际环境条件偏差，最大限度模拟土壤环境条件，利于准确描述土壤水分运动过程和研究作物蒸腾耗水规律；通过小型原位蒸渗仪与智能灌溉系统结合，能最大程度模拟作物栽培条件和稳定土壤水分下实际蒸散量

PROKARYOTIC EXPRESSION AND IDENTIFICATION OF ALLOPHYCOCYANIN α SUBUNIT GENE FROM PORPHYRA HAITANENSIS

通过PCR的方法从重组质粒pMD-apcAB中扩增坛紫菜别藻蓝蛋白α亚基基因(apcA),并将其克隆到高效表达外源基因的原核表达质粒pTO-T7。将构建好的质粒导入表达型大肠杆菌BL21(DE3),IPTG诱导表达,并对表达产物进行Western-blot和质谱鉴定。结果显示:apcA全长486bp,表达的α亚基(apcA)为带有原核表达载体T7g10的12个起始氨基酸的融合蛋白,其分子量约为19.7KD。0.5mmol/L的IPTG在37℃诱导6h时,apcA的表达量达到最大,达菌体总蛋白50%以上。Western-blot和质谱鉴定的结果表明获得的融合蛋白为重组坛紫菜别藻蓝蛋白α亚基。Allophycocyanins(APC) consist of α and β subunits,was one of phycobiliproteins,act as substances of light-havesting and transferring energy to photosystem reaction centers in algal photosynthesis;it also as a kind of bioactive substances applied perspective in quite a lot of fields.Although the apcA and apcB genes encoding allophycocyanin α and β subunits of Cyanophora paradoxa,Anabaena variabilis,Cyanidium caldarium,Synechocystis 6714 and Aglaothamnion neglectum(Rhodophyta) were also cloned,the research related to apc genes in macro-alga has not been reported.In this study,the apcA gene of Porphyra haitanensis was PCR amplified from pMD-apcAB recombinant plasmid and cloned into E.coli fusion expression pTO-T7 vector which allows the overexpression of a target protein.The recombinat plasmid pTO-T7-apcA was transformed into E.coli BL21(DE3) and induced in 0.5mmol/L IPTG in 37℃,the induce product was identified by western blotting and mass spectrum.The results showed that the 486bp sequence of apcA was successfully inserted into pTO-T7 plasmid.SDS-PAGE analysis of the inclusion of E.coli carrying pTO-T7-apcA showed a band with molecular mass of 19.7KD in agreement with a fusion APC α protein with the first 12 Nterminaminol amino acids of T7g10, which was identical to what had been anticipated.And the recombinant fusion protein accounted for more than 50% of the total E.coli protein after 6 hours inducing.The result of western blotting confirmed that the recombinant fusion protein could specifically react with antibody against native APC proteins.And the mass spectrum results proved that the target protein was allophycocyanin α subunit of Porphyra haitanensis.福建省重大农业科技项目(2001Z017);; 国家海洋863项目(2002AA603023)资