气吸式覆膜精量油菜播种机排种性能试验与优化设计

针对目前高寒地油菜播种机普遍存在的重播漏播率高、人工劳动强度大、生长期缺水等问题，研究设计了一种气吸式精量播种机，一次性完成膜上播种、施肥、滴水灌溉、覆膜。分析了播种机主要结构、工作原理，对其关键部件进行结构设计，以排种盘转速、气吸室负压、排种盘型孔直径为试验因素，利用软件优化分析获得合理参数组合。结果表明：播种机排种盘转速197 r·min^-1、气吸室负压2.5 kPa、排种盘型孔直径1.2 mm时，田间播种合格率为93%、重播率3%、漏播率1%，播种质量较好。田间试验表明上述参数组合下排种器工作性能满足油菜播种机工作性能要求，该研究为油菜精密播种机的研究和设计提供了理论和技术参数。     

智慧图书馆微观知识生态系统运行机理研究

伴随多元化时代的来临,用户的知识需求日益多元化、专业化,对图书馆服务提出了新的挑战。对智慧图书馆微观知识生态系统运行机理的研究,能够为新型知识服务提供理论基础,保障知识资源进行有效的优化整合,实现服务升级。文章在简要分析智慧图书馆微观知识生态系统四大要素的基础上,着重从社会发展、技术进步,知识富集、优化调整和需求驱动、服务升级三方面探讨其形成动因,重点分析智慧图书馆微观知识生态系统的生命周期,最后从合作、循环和保障三方面探讨其运行机理。     

黑龙江省农产品深加工产业发展现状与对策

黑龙江省的农产品加工体系已经初步形成，但农业发展主要依赖于“原”字号产品。阐述了黑龙省农产品深加工产业建设存在的问题，通过分析制约农产品深加工产业发展的主要原因，从优化种植结构、整合现有资源、拓宽农产品销路以及提高农产品附加值4个方面提出解决对策。旨在做强食品加工业，上调农产品利润空间，通过“大龙头、大链条、大产业、大品牌的高效农业全产业链”促进粗放农产品向高附加值产品的转变，努力实现从产粮大省到农业强省的新跨越。      

漆酶LAC表达与鸭梨果心褐变的关系

【目的】探究在不同成熟度和降温贮藏方式下,LAC表达模式与鸭梨果心褐变的关系,为进一步解析鸭梨果心褐变机制提供理论依据。【方法】以鸭梨作为材料,通过对不同成熟度（早采、中采和晚采）的鸭梨进行急速降温（急降）和缓慢降温（缓降）处理,观察贮藏期间鸭梨果心褐变情况,测定漆酶（Laccase,LAC）活性及其基因LAC的相对表达量,研究LAC在鸭梨果心褐变过程中的参与作用。【结果】冷藏60 d时,晚采鸭梨出现褐变,晚采缓降处理的鸭梨果心褐变指数为0.32,是同期急速降温处理的2.56倍;在贮藏90 d时,中采缓降处理的褐变指数是0.24,中采急降处理的褐变指数仅为0.01。各个处理组在贮藏期间LAC活性多数表现为先逐渐升高后下降的趋势,晚采的果实在贮藏60 d时出现活性高峰,褐变发生;早采和中采鸭梨LAC活性高峰均在90 d时出现,褐变程度低于晚采鸭梨。在贮藏期间,缓慢降温处理的LAC活性高于急速降温处理。鸭梨LAC14和LAC7表达量呈先上升后下降的趋势,LAC6表现为先下降后上升再降低的变化趋势;中采、晚采鸭梨在贮藏60 d时,LAC14和LAC7表达量最高。【结论】与缓慢降温相比,急速降温处理减少了鸭梨果心褐变的发生。在整个贮藏期间,LAC活性呈先上升后下降然后又上升的趋势,其峰值时的活性高低次序为：晚采>中采>早采,这与果心褐变趋势一致;LAC在鸭梨果心褐变过程中上调表达。相比缓慢降温处理,急速降温处理具有较低的LAC7、LAC14和LAC6表达量。急速降温结合适时采收能够抑制LAC的上调表达,减少鸭梨果心褐变发生。     

植物免疫诱导剂在草莓中的应用情况

为了助力实现草莓的安全生产,对一类能诱导植物产生免疫防御反应的植物免疫诱导剂在草莓中的应用情况进行综述。主要阐述了植物免疫诱导剂的种类、诱导机理及其在草莓栽培上的应用现状,发现:植物免疫诱导剂能促进草莓生长和发育、诱导抗病性、提高产量、改善果实品质、提高耐贮性等,从而减少了化学农药的使用,有利于草莓高质量生产,应用前景广阔。     

耕作方式及秸秆还田对土壤性质、微生物碳源代谢及小麦产量的影响

以小麦品种济麦22为试验材料,采用裂区试验设计,耕作方式为主区,分别设常规翻耕(C)、深松(S)、旋耕(R)处理,副区为秸秆还田量,分别设秸秆全还田(P)和秸秆不还田(A)处理,采用Biolog Eco技术测定土壤微生物碳源代谢功能,并分析土壤基本理化性质和作物产量。结果显示:深松与秸秆还田均有利于土壤含水量和有机碳含量的提高,0～15 cm土层分别提高了9.78%和24.00%,15～30 cm土层分别提高了7.08%和15.81%;深松提高了15～30 cm土层的pH值6.67%,秸秆还田提高了0～15 cm土层的pH值4.32%。深松和秸秆还田均有利于代谢多样性(丰富度指数、香浓多样性指数)、碳源代谢强度的提高,0～15 cm土层分别提高了26.84%、3.84%和38.02%,15～30 cm土层分别提高了11.87%、 3.63%和14.74%。主成分分析表明常规翻耕秸秆不还田和旋耕耕作秸秆不还田碳源代谢功能相近,15～30 cm层次内常规翻耕秸秆全还田碳源代谢功能和深松耕作秸秆全还田处理相近。深松和秸秆还田平均提高了小麦产量5.82%,微生物碳源代谢功能与小麦产量具有极显著的相关性。     

生物炭对Bt Cry1Ac蛋白抗紫外能力影响

为了研究生物炭对紫外线的防护作用，以豆壳烧制的生物炭作为载体，研究生物炭对Bt Cry1Ac蛋白的吸附行为以及生物炭对Cry1Ac蛋白的紫外保护作用。使用扫描电子显微镜、透射电子显微镜、X-射线粉末衍射以及傅立叶红外光谱等手段对生物炭的形貌和结构进行表征。结果表明，生物炭是典型的多孔结构材料，表面具有丰富的官能团。Cry1Ac蛋白与生物炭吸附平衡时间为50 min，最合适的吸附浓度比（生物炭：蛋白）为1：100，二者吸附符合准二级动力学模型和Langmuir模型。在UVB紫外照射4 h后，生物炭与Cry1Ac蛋白复合物对棉铃虫的生物活性是单纯蛋白的4.93倍，显示生物炭具有较好的紫外抵抗效果。研究结果初步表明，制备得到的生物炭能够显著提高Cry1Ac蛋白的抗紫外能力，为后续研发耐受紫外线的农药剂型提供新材料。     

The M43 domain-containing metalloprotease RcMEP1 in Rhizoctonia cerealis is a pathogenicity factor during the fungus infection to wheat

Wheat(Triticum aestivum L.) is an important staple crop for global human. The necrotrophic fungus Rhizoctonia cerealis is the causal pathogen of sharp eyespot, a devastating disease of wheat. Herein, we identified RcMEP1, a zinc metalloproteaseencoding gene from R. cerealis genomic sequences, and characterized its pathogenesis function. RcMEP1 expressed at markedly-high levels during R. cerealis infection process to wheat. The predicted protein RcMEP1 comprises of 287 amino acid residues and contains a signal peptide and a M43 metalloprotease domain harboring the active site motif(HEVGHWLGLYH). The assays of Agrobacterium tumefaciens-mediated transient expression in Nicotiana benthamiana leaves indicated that RcMEP1 is an apoplastic elicitor of cell death, and that the predicted signal peptide functions and is required for secretion and cell death-induction. The purified RcMEP1 protein and its M43 domain peptide were individually able to induce plant cell death and H2 O2 accumulation, and to inhibit expression of host chitinases when infiltrated into wheat and N. benthamiana leaves, while the M43 domain-deleting peptide and negative control lacked the capacity. Moreover, compared with the control pretreatment, the purified RcMEP1 protein or its M43-domain peptide resulted in enhanced pathogenesis in the inoculated wheat, whereas the M43 domain-deleting peptide failed. These results suggest that RcMEP1 acted as an important pathogenicity factor during R. cerealis infection to wheat and that its signal peptide and M43 domain are required for the secretion and pathogenesis of RcMEP1. This study provides insights into pathogenesis role of M43 domain-containing metalloproteases during R. cerealis infection to wheat.     

南海大顶苦瓜规范化栽培技术

为了发挥广东省佛山市的传统特色蔬菜——大顶苦瓜的产品优势,提高农户的规范化栽培技术水平,在改良南海大顶苦瓜品种的基础上,制定出配套的规范化栽培技术措施,内容包括品种特性、产地环境要求、育苗、田间管理措施和采收,旨在进一步提高南海大顶苦瓜的生产效益,大力推广这一传统特色蔬菜品种。     

MicroRNA-145 inhibits epithelial-mesenchymal transition in human renal cancer A-498 cells by ADAM28

AIM: To investigate the inhibitory effect of microRNA-145 (miR-145) on epithelial-mesenchymal transition (EMT) in renal cancer A-498 cells. METHODS: The A-498 cells were transfected with miR-145 mimics (M145) and mimic negative control(MNC), which served as M145 group and MNC group, respectively. Mock control (MC) group was set up using untreated A-498 cells. The expression level of miR-145 in each group was detected by RT-qPCR. Transwell assay was used to detect the invasion ability of the cells. The protein expression of vimentin, E-cadherin and ADAM28 was determined by Western blot. Bioinformatic method was used to predict the target genes of miR-145. Antagonistic effect of ADAM28 over-expression on the inhibition of EMT by miR-145 was detected by Western blot. The relationship between miR-145 and ADAM28 was analyzed by dual-luciferase reporter assay. RESULTS: The expression level of miR-145 in M145 group was significantly up-regulated than that in MC group (P<0.05). The number of invasive cells in M145 group was 12.78±3.37, which was significantly lower than that in MC group (P<0.05). ADAM28 may be the target gene of miR-145. Compared with MC group, the protein expression of vimentin and ADAM28 in M145 group was significantly decreased (P<0.05), while the protein expression of E-cadherin was significantly increased (P<0.05).After ADAM28 over-expression, the protein expression of vimentin in the A-498 cells of M145 group was significantly increased (P<0.05), and the protein expression of E-cadherin was significantly decreased (P<0.05). The results of dual-lucife-irasei reporter assay showed that ADAM28 was a downstream target gene of miR-145. CONCLUSION: miR-145 may inhibit the expression of EMT-related proteins through the downstream target gene ADAM28 and inhibit the EMT process of renal cancer A-498 cells.