The effect of calcium chloride injection on shear force and caspase activities in bovine longissimus muscles during postmortem conditioning

Tenderness is considered as the most important quality determinant of meat. Calcium chloride application has been shown to improve tenderness by regulating endogenous proteinases. This study was designed to determine the effect of 300 mM calcium chloride injection on myofibrillar structures, caspase activities and shear force in longissimus muscles of bulls during postmortem storage of 7 days. Myofibrillar fragmentation index was determined as an index of proteolysis occurring in muscle fibers and associated proteins. Maximum tenderness was observed at days 4 and 7 in both treated and control samples. The injection of calcium chloride significantly increased myofibrillar proteolysis and improved tenderness at postmortem days 4 and 7. The treatment reduced caspase-9 activity at 4 h and day 4, whereas those of caspase-8 and -3 activities at days 1 and 4 with respect to control. The improved tenderness and increased myofibril fragmentation with decreased caspase activities suggested that the proteolytic systems activated with calcium chloride injection possibly behave independent of the caspase system.     

基于主成分-聚类-逐步回归分析构建番茄苗期耐铝性综合评价体系

铝毒是限制酸性土壤中作物产量的主要因素之一。番茄(Solanum lycopersicum)是适合在酸性土壤中种植的主要经济作物, 不同品种番茄对铝胁迫的响应存在差异, 因此, 筛选苗期耐铝毒种质对番茄生产及研究具有重要意义。以10个番茄品种为材料, 采用室内土培盆栽, 设置1 000 µmol∙L^-1 AlCl₃·6H₂O处理, 测定反映植物铝胁迫下生长状况的16个形态、生理生化及光合指标。通过主成分分析, 将铝胁迫下番茄幼苗的16个指标转化为5个独立的综合指标, 累积贡献率达90.779%。基于耐铝性综合评价值(A)的系统聚类分析, 将供试种质划分为5类, 第I类为高度耐铝品种Qianxi, 第V类为高度不耐铝品种Puluowangsi。经多元线性逐步回归分析得出番茄苗期耐铝评价方程: y=0.046+0.405X₆+0.515X₁₀-0.207X₁₅+0.028X₃ (R²=0.997), 从16个指标中提取出与A值显著相关(P<0.01)的4个指标: 丙二醛含量(X₃)、净光合速率(X₆)、叶面积(X₁₀)和地下部干重(X₁₅)。利用评价方程可判断不同番茄品种苗期的耐铝性, 使番茄耐铝性鉴定工作快速简便。     

Separation and detection of vitellogenin in fish plasma by capillary zone electrophoresis

A method for coupling capillary zone electrophoresis (CZE) with rapid membrane chromatography purification (RMCP) was established for the analysis of vitellogenin (VTG) in male fish plasma induced with 17ss-estrodiol. CZE analyses of purified VTG were performed in a buffer containing 25 mM sodium borate (pH 8.4). A 50 microm i.d. fused-silica capillary was used for separation and the detection was carried out by UV-diode array at 214 nm. Inter- and intra-assay variabilities of the proposed method were less than 10.06 and 1.95%, respectively. The method has good linear relationship over the scope of 15-2250 microg/ml with a correlation coefficient of R2 = 0.9965 and a detection limit of 7.0 microg/ml. The established CZE method was also applied to directly separate and identify VTG from fish plasma. The results indicated this method could minimize interferences from plasma proteins, allowing the detection of at least 62.5 microg/ml of VTG proteins in total proteins. This is a rapid and easy method to determine the quantity and purity of VTG compared to Bradford method and SDS-PAGE.     

Efficient Editing of an Adenoviral Vector Genome with CRISPR/Cas9

Immunotherapy based on genetic modification of T cells has played an important role in the treatment of tumors and viral infections. Moreover, adenoviral vectors engineered with improved safety due to their inability to integrate into the host genome have been key in the clinical application of T cell therapy. However, the commonly used adenoviral vector Ad5 exhibits low efficiency of infection of human T cells and the details of the intracellular trafficking pathway of adenoviral vectors in human primary T cells remains unclear. Resolution of these issues will depend on successful modification of the adenoviral vector. To this end, here we describe the successful establishment of a simple and efficient method for editing adenoviral vectors in vitro using the CRISPR-Cas9 gene editing system to target the adenoviral fiber gene. Electronic supplementary materialThe online version of this article (10.1007/s12088-020-00905-3) contains supplementary material, which is available to authorized users.     

Photosynthetic electron flow affects H2O2 signaling by inactivation of catalase in Chlamydomonas reinhardtii

A specific signaling role for H₂O₂ in Chlamydomonas reinhardtii was demonstrated by the definition of a promoter that specifically responded to this ROS. Expression of a nuclear-encoded reporter gene driven by this promoter was shown to depend not only on the level of exogenously added H₂O₂ but also on light. In the dark, the induction of the reporter gene by H₂O₂ was much lower than in the light. This lower induction was correlated with an accelerated disappearance of H₂O₂ from the culture medium in the dark. Due to a light-induced reduction in catalase activity, H₂O₂ levels in the light remained higher. Photosynthetic electron transport mediated the light-controlled down-regulation of the catalase activity since it was prevented by 3-(3′4′-dichlorophenyl)-1,1-dimethylurea (DCMU), an inhibitor of photosystem II. In the presence of light and DCMU, expression of the reporter gene was low while the addition of aminotriazole, a catalase inhibitor, led to a higher induction of the reporter gene by H₂O₂ in the dark. The role of photosynthetic electron transport and thioredoxin in this regulation was investigated by using mutants deficient in photosynthetic electron flow and by studying the correlation between NADP-malate dehydrogenase and catalase activities. It is proposed that, contrary to expectations, a controlled down-regulation of catalase activity occurs upon a shift of cells from dark to light. This down-regulation apparently is necessary to maintain a certain level of H₂O₂ required to activate H₂O₂-dependent signaling pathways.