利用光合细菌进行微生物修复：一种降低辛硫磷在养殖水中积累的低成本方法

【背景】中国是农业生产大国,渔林农牧占比庞大。有机农药无论在畜牧业还是水产养殖业都有广泛的应用。有机磷农药(Organophosphorus Pesticide,OP)是应用最广泛的有机农药,具有低毒和不易残留的优点。OP在水体中大量积累可通过生物富集作用间接影响人体健康,由此产生的生殖毒性不容忽视。光合细菌作为环境友好型水体有益菌,部分菌种具有降解有机农药的功能。【目的】自上海海洋大学明湖中分离纯化得到一株光合细菌(编号SPZ)。探究其对辛硫磷的耐受程度及降解效果,为养殖水体中有机磷农药的生物降解提供目的菌株。【方法】利用16S rRNA基因序列分析方法对目标菌株进行种属鉴定;利用紫外分光光度法测定分离菌株SPZ和标准菌株ST在不同接种量下的OD660并测定实验周期内光合细菌在不同浓度辛硫磷中OD660的变化趋势,以示辛硫磷对光合细菌的毒性作用;利用高效液相色谱法(High Performance Liquid Chromatography,HPLC)测定菌株对水体辛硫磷的降解能力;通过HPLC测定加热致死菌与活菌对水体辛硫磷的降解能力,确定菌株对辛硫磷的降解方式。【结果】16S r...     

梨果黑斑病菌AaCaMK基因克隆、生物信息学分析及其在侵染结构分化中的表达分析

[背景] 钙/钙调素依赖型蛋白激酶（Calcium/Calmodulin-Dependent Protein Kinase,CaMK）是真核生物细胞钙信号途径中钙调素下游的一类重要靶蛋白,对病原物生长、胁迫响应及致病性等具有重要的调控作用。[目的] 对梨果黑斑病菌互隔交链孢（Alternaria alternata）AaCaMK基因进行克隆、生物信息学分析,并对其在侵染结构分化过程中的基因表达情况进行分析,为进一步研究梨果黑斑病菌钙离子信号途径中AaCaMK对A.alternata侵染结构分化调控的分子机制提供一定的理论依据。[方法] 采用同源克隆法从A. alternata JT-03中克隆得到3个AaCaMK基因;通过TMHMM、ProtScale、SOPMA等软件对AaCaMK基因进行生物信息学分析;利用实时荧光定量PCR （RT-qPCR）技术分析AaCaMK在梨果黑斑病菌侵染结构分化过程中的表达情况。[结果] 克隆得到片段分别为1 212、1 200、2 349 bp的AaCaMK1、AaCaMK2和AaCaMK3基因;生物信息学分析表明,AaCaMK1、AaCaMK2和AaCaMK3均含有典型的蛋白激酶超家族催化结构域（PKC_Like Superfamily）,并且AaCaMK1和AaCaMK2共同含有CaMK类丝/苏氨酸蛋白激酶催化结构域（STKc_CaMK）,AaCaMK3含有LKB1/CaMKK类丝/苏氨酸蛋白激酶催化结构域（STKc_LKB1_CaMKK）;同源性分析表明,AaCaMK1、AaCaMK2和AaCaMK3分别与玉米大斑病菌CAK1、CAK2和CAK3的相似性高达94.32%、97.49%和86.57%;RT-qPCR分析表明,AaCaMK1、AaCaMK2和AaCaMK3在疏水及果蜡诱导A. alternata侵染结构分化过程中均显著上调表达（P<0.05）,而且果蜡诱导作用更显著。其中AaCaMK1和AaCaMK2在附着胞形成时期（6 h）表达量为对照的1.51倍和3.05倍,而AaCaMK3在侵染菌丝形成阶段（8 h）表达量最高,为对照的2.86倍,并且在果蜡诱导下,这3个基因在芽管伸长阶段（4 h）的上调表达量显著高于疏水界面。[结论] 钙信号中AaCaMK基因在疏水及果蜡诱导A.alternata侵染结构分化过程中发挥重要的调控作用。     

产小檗碱内生真菌的诱变

以产小檗碱的内生真菌S6为出发菌株,采用多种单一或复合诱变措施对其菌丝体进行诱变处理,最终筛选得到高产菌株S-NU-302。其小檗碱产量比出发菌株提高170%,达到12.28 mg/L;生长速率提高81.7%,达到5.72 g/L;经10次传代显示该菌株具有良好的遗传稳定性。     

中国黑木耳主要栽培菌株ISSR指纹分析及SCAR标记

采用ISSR标记技术对来自全国的黑木耳34个主要栽培菌株进行DNA指纹分析,初步构建其标准化DNA指纹图谱;在ISSR指纹分析基础上进行聚类分析,并将黑木耳两个栽培菌株173和186中扩增获得的ISSR特异性DNA带转化为可以直接用于菌株快速鉴定的SCAR标记.研究表明,我国黑木耳栽培菌株遗传背景差异不大,存在同物异名现象,而采用ISSR指纹及其SCAR标记鉴定黑木耳栽培菌株具有重要意义.     

Barley GRIK1‐SnRK1 kinases subvert a viral virulence protein to upregulate antiviral RNAi and inhibit infection

Viruses often usurp host machineries for their amplification, but it remains unclear if hosts may subvert virus proteins to regulate viral proliferation. Here, we show that the 17K protein, an important virulence factor conserved in barley yellow dwarf viruses (BYDVs) and related poleroviruses, is phosphorylated by host GRIK1‐SnRK1 kinases, with the phosphorylated 17K (P17K) capable of enhancing the abundance of virus‐derived small interfering RNAs (vsiRNAs) and thus antiviral RNAi. Furthermore, P17K interacts with barley small RNA‐degrading nuclease 1 (HvSDN1) and impedes HvSDN1‐catalyzed vsiRNA degradation. Additionally, P17K weakens the HvSDN1‐HvAGO1 interaction, thus hindering HvSDN1 from accessing and degrading HvAGO1‐carried vsiRNAs. Importantly, transgenic expression of 17K phosphomimetics (17K^5D), or genome editing of SDN1, generates stable resistance to BYDV through elevating vsiRNA abundance. These data validate a novel mechanism that enhances antiviral RNAi through host subversion of a viral virulence protein to inhibit SDN1‐catalyzed vsiRNA degradation and suggest new ways for engineering BYDV‐resistant crops.     

Long noncoding RNA lncMREF promotes myogenic differentiation and muscle regeneration by interacting with the Smarca5/p300 complex

Long noncoding RNAs (lncRNAs) play important roles in the spatial and temporal regulation of muscle development and regeneration. Nevertheless, the determination of their biological functions and mechanisms underlying muscle regeneration remains challenging. Here, we identified a lncRNA named lncMREF (lncRNA muscle regeneration enhancement factor) as a conserved positive regulator of muscle regeneration among mice, pigs and humans. Functional studies demonstrated that lncMREF, which is mainly expressed in differentiated muscle satellite cells, promotes myogenic differentiation and muscle regeneration. Mechanistically, lncMREF interacts with Smarca5 to promote chromatin accessibility when muscle satellite cells are activated and start to differentiate, thereby facilitating genomic binding of p300/CBP/H3K27ac to upregulate the expression of myogenic regulators, such as MyoD and cell differentiation. Our results unravel a novel temporal-specific epigenetic regulation during muscle regeneration and reveal that lncMREF/Smarca5-mediated epigenetic programming is responsible for muscle cell differentiation, which provides new insights into the regulatory mechanism of muscle regeneration.     

DAZL regulates proliferation of human primordial germ cells by direct binding to precursor miRNAs and enhances DICER processing activity

Understanding the molecular and cellular mechanisms of human primordial germ cells (hPGCs) is essential in studying infertility and germ cell tumorigenesis. Many RNA-binding proteins (RBPs) and non-coding RNAs are specifically expressed and functional during hPGC developments. However, the roles and regulatory mechanisms of these RBPs and non-coding RNAs, such as microRNAs (miRNAs), in hPGCs remain elusive. In this study, we reported a new regulatory function of DAZL, a germ cell-specific RBP, in miRNA biogenesis and cell proliferation. First, DAZL co-localized with miRNA let-7a in human PGCs and up-regulated the levels of >100 mature miRNAs, including eight out of nine let-7 family, miR21, miR22, miR125, miR10 and miR199. Purified DAZL directly bound to the loops of precursor miRNAs with sequence specificity of GUU. The binding of DAZL to the precursor miRNA increased the maturation of miRNA by enhancing the cleavage activity of DICER. Furthermore, cell proliferation assay and cell cycle analysis confirmed that DAZL inhibited the proliferation of in vitro PGCs by promoting the maturation of these miRNAs. Evidently, the mature miRNAs up-regulated by DAZL silenced cell proliferation regulators including TRIM71. Moreover, DAZL inhibited germline tumor cell proliferation and teratoma formation. These results demonstrate that DAZL regulates hPGC proliferation by enhancing miRNA processing.     

CRISPR/Cas9-induced structural variations expand in T lymphocytes in vivo

CRISPR/Cas9 has been adapted to disrupt endogenous genes in adoptive T-lymphocyte therapy to prevent graft-versus-host disease. However, genome editing also generates prevalent deleterious structural variations (SVs), including chromosomal translocations and large deletions, raising safety concerns about reinfused T cells. Here, we dynamically monitored the progression of SVs in a mouse model of T-cell receptor (TCR)-transgenic T-cell adoptive transfer, mimicking TCR T therapeutics. Remarkably, CRISPR/Cas9-induced SVs persist and undergo clonal expansion in vivo after three weeks or even two months, evidenced by high enrichment and low junctional diversity of identified SVs post infusion. Specifically, we detected 128 expanded translocations, with 20 615 as the highest number of amplicons. The identified SVs are stochastically selected among different individuals and show an inconspicuous locus preference. Similar to SVs, viral DNA integrations are routinely detected in edited T cells and also undergo clonal expansion. The persistent SVs and viral DNA integrations in the infused T cells may constantly threaten genome integrity, drawing immediate attention to the safety of CRISPR/Cas9-engineered T cells mediated immunotherapy.     

The Heterogeneity in the Landscape of Gene Dominance in Maize is Accompanied by Unique Chromatin Environments

Subgenome dominance after whole-genome duplication (WGD) has been observed in many plant species. However, the degree to which the chromatin environment affects this bias has not been explored. Here, we compared the dominant subgenome (maize1) and the recessive subgenome (maize2) with respect to patterns of sequence substitutions, genes expression, transposable element accumulation, small interfering RNAs, DNA methylation, histone modifications, and accessible chromatin regions (ACRs). Our data show that the degree of bias between subgenomes for all the measured variables does not vary significantly when both of the WGD genes are located in pericentromeric regions. Our data further indicate that the location of maize1 genes in chromosomal arms is pivotal for maize1 to maintain its dominance, but location has a less effect on maize2 homoeologs. In addition to homoeologous genes, we compared ACRs, which often harbor cis-regulatory elements, between the two subgenomes and demonstrate that maize1 ACRs have a higher level of chromatin accessibility, a lower level of sequence substitution, and are enriched in chromosomal arms. Furthermore, we find that a loss of maize1 ACRs near their nearby genes is associated with a reduction in purifying selection and expression of maize1 genes relative to their maize2 homoeologs. Taken together, our data suggest that chromatin environment and cis-regulatory elements are important determinants shaping the divergence and evolution of duplicated genes.