LRP6 downregulation promotes cardiomyocyte proliferation and heart regeneration

The adult mammalian heart is thought to be a terminally differentiated organ given the postmitotic nature of cardiomyocytes. Consequently, the potential for cardiac repair through cardiomyocyte proliferation is extremely limited. Low-density lipoprotein receptor-related protein 6 (LRP6) is a Wnt co-receptor that is required for embryonic heart development. In this study we investigated the role of LRP6 in heart repair through regulation of cardiomyocyte proliferation. Lrp6 deficiency increased cardiomyocyte cell cycle activity in neonatal, juvenile and adult mice. Cardiomyocyte-specific deletion of Lrp6 in the mouse heart induced a robust regenerative response after myocardial infarction (MI), led to reduced MI area and improvement in left ventricular systolic function. In vivo genetic lineage tracing revealed that the newly formed cardiomyocytes in Lrp6-deficient mouse hearts after MI were mainly derived from resident cardiomyocytes. Furthermore, we found that the pro-proliferative effect of Lrp6 deficiency was mediated by the ING5/P21 signaling pathway. Gene therapy using the adeno-associated virus (AAV)9 miRNAi-Lrp6 construct promoted the repair of heart injury in mice. Lrp6 deficiency also induced the proliferation of human induced pluripotent stem cell-derived cardiomyocytes (iPSC-CMs). Our study identifies LRP6 as a critical regulator of cardiomyocyte proliferation, which may lead to the development of a novel molecular strategy to promote myocardial regeneration and repair.Subject terms: Cell-cycle exit, Cytokinesis     

橘小实蝇成虫肠道可培养细菌群落结构分析

【目的】研究橘小实蝇(Bactrocera dorsalis) 3个种群(实验室正常喂养种群、实验室无菌糖水喂养种群和野生种群)成虫肠道可培养细菌的群落结构组成。【方法】利用16S rRNA基因的聚合酶链式反应-变性梯度凝胶电泳(PCR-DGGE)分析技术,结合菌落形态观察和生理生化特征鉴定细菌种类。【结果】从橘小实蝇3个种群成虫肠道600株可培养细菌得到53种不同细菌遗传型,分属于肠杆菌科(Enterobacteriaceae)、肠球菌科(Enterococcaceae)和芽孢杆菌科(Bacillaceae)等3个科。其中肠杆菌科是肠道可培养细菌最优势的细菌种类。同样以序列相似性大于97%的菌株归为相同的细菌种类为标准,找到了橘小实蝇3个种群可培养细菌的共有菌种,结合菌落形态观察和生理生化特征鉴定,确定共有菌种为肠杆菌属5株,克雷伯氏菌属2株,柠檬酸杆菌属1株,泛菌属1株,肠球菌属2株,以及芽孢杆菌属4株。【结论】通过研究橘小实蝇成虫肠道可培养细菌群落结构组成,可为探讨肠道菌群对寄主的生理功能和生态学意义奠定基础,最终为利用微生物防治此类害虫提供新思路。     

我国甜菜夜蛾间歇性暴发的非均衡性循环波动

[摘要] 为进一步了解我国甜菜夜蛾Spodoptera exigua ( Hbner)间歇性暴发成灾的规律,作者应用时间序列分析技术研究了我国甜菜夜蛾间歇性暴发的时间序列波动规律。结果表明,在1949—2008年的60a中,我国甜菜夜蛾大尺度暴发总年频次为120次,各年度暴发次数(年频次)存在着非均衡性循环波动特征,并且在其波动过程中呈明显的上升趋势。按“年频次”强度,可将我国1949—2008年60a中甜菜夜蛾发生过程,划分成两个明显不同的阶段。第一阶段（1949—1984年）为平稳低发阶段,36a总年频次量为4次,年平均仅0.11次;第二阶段（1985—2008年）则为波浪式上升性高发阶段,24a总年频次为116次,年平均4.83次（为第一阶段的43.91倍））。按第二阶段24a（1985—2008）数据进行自相关系数和频谱图分析,结果表明,我国甜菜夜蛾大尺度暴发存在2.8a和11.2a2种不同长度的循环周期,其暴发趋势指数对滞后1a和滞后4a的影响为正相关,而对滞后5a和滞后6a的影响则为负相关。本文根据甜菜夜蛾暴发指数的非均衡周期性特征,建立了以时间序列为自变量的甜菜夜蛾暴发指数非均衡周期性预测模型,经回代结果检验,理论值与实测值之间无显著差异。     

转Bt水稻土壤跳虫群落组成及其数量变化

以转Bt水稻恢复系"克螟稻"(Cry1Ab纯合基因型)和"华恢1号"(Cry1Ab+Cry1Ac融合基因型)以及融合基因型转Bt水稻杂交系"Bt汕忧63",及其对照亲本水稻"秀水11"、"明恢63"和"汕优63"稻田土壤跳虫类群为对象,系统研究转Bt水稻种植下土壤跳虫群落组成及其数量动态变化,以评价不同基因型和不同育种品系转Bt水稻种植下稻田土壤生态安全性。结果表明,转Bt水稻种植导致土壤跳虫个别稀有类群的消失,并显著影响半土生和真土生类群以及土壤跳虫总量,但对群落多样性、均匀度和种类丰富度等影响不显著。与对照亲本相比,Cry1Ab转Bt稻田半土生类群和土壤跳虫总量及其种类丰富度指标显著增加了54.7%、44.4%和26.7%;Cry1Ab+Cry1Ac转Bt杂交稻田球角跳属百分比和真土生跳虫数量显著增加了212.3%和180.4%。就恢复系处理而言,与Cry1Ab转Bt水稻相比,Cry1Ab+Cry1Ac转Bt水稻种植导致棘跳属、球角跳属和原等跳属百分比以及半土生跳虫数量分别显著降低了62.1%、56.7%、61.8%和43.4%,同时,显著提高了裔符跳属百分比达88.2%。就Cry1Ab+Cry1Ac融合基因型转Bt水稻而言,与恢复系相比,转Bt杂交稻种植导致球角跳属和原等跳属百分比,半土生类群和土壤跳虫总量及其种类丰富度和群落多样性显著增加了312.9%和171.6%,302.4%和233.2%,以及54.0%和26.7%,同时,显著降低了裔符跳属百分比达65.5%。     

谷氨酸棒杆菌L-天冬氨酸α-脱羧酶在大肠杆菌中的表达及酶转化生产β-丙氨酸

【目的】克隆谷氨酸棒杆菌来源L-天冬氨酸α-脱羧酶基因, 实现其在大肠杆菌中的异源表达, 并进行酶转化L-天冬氨酸合成β-丙氨酸的研究。【方法】PCR扩增谷氨酸棒杆菌L-天冬氨酸α-脱羧酶基因pand, 构建表达载体pET24a(+)-Pand, 转化宿主菌大肠杆菌BL21(DE3), 对重组菌进行诱导表达, 表达产物经DEAE离子交换层析和G-75 分子筛层析纯化后进行酶学性质研究, 然后进行酶转化实验, 说明底物和产物对酶转化的影响。【结果】重组菌SDS-PAGE分析表明Pand表达量可达菌体总蛋白的50%以上, AccQ·Tag法检测酶活达到94.16 U/mL。该重组酶最适反应温度为55 °C, 在低于37 °C时保持较好的稳定性, 最适pH为6.0, 在pH 4.0?7.0范围内有较好的稳定性。酶转化实验说明: 底物L-天冬氨酸和产物β-丙氨酸对转化反应均有抑制作用; 实验建立了较优的酶转化反应方式, 在加酶量为每克天冬氨酸3 000 U时, 以分批加入固体底物L-天冬氨酸的形式, 使100 g/L底物转化率达到97.8%。【结论】重组L-天冬氨酸α-脱羧酶在大肠杆菌中获得高效表达, 研究了酶转化生产β-丙氨酸的影响因素, 为其工业应用奠定了基础。     

mTORC1-independent translation control in mammalian cells by methionine adenosyltransferase 2A and S-adenosylmethionine

Methionine adenosyltransferase (MAT) catalyzes the synthesis of S-adenosylmethionine (SAM). As the sole methyl-donor for methylation of DNA, RNA, and proteins, SAM levels affect gene expression by changing methylation patterns. Expression of MAT2A, the catalytic subunit of isozyme MAT2, is positively correlated with proliferation of cancer cells; however, how MAT2A promotes cell proliferation is largely unknown. Given that the protein synthesis is induced in proliferating cells and that RNA and protein components of translation machinery are methylated, we tested here whether MAT2 and SAM are coupled with protein synthesis. By measuring ongoing protein translation via puromycin labeling, we revealed that MAT2A depletion or chemical inhibition reduced protein synthesis in HeLa and Hepa1 cells. Furthermore, overexpression of MAT2A enhanced protein synthesis, indicating that SAM is limiting under normal culture conditions. In addition, MAT2 inhibition did not accompany reduction in mechanistic target of rapamycin complex 1 activity but nevertheless reduced polysome formation. Polysome-bound RNA sequencing revealed that MAT2 inhibition decreased translation efficiency of some fraction of mRNAs. MAT2A was also found to interact with the proteins involved in rRNA processing and ribosome biogenesis; depletion or inhibition of MAT2 reduced 18S rRNA processing. Finally, quantitative mass spectrometry revealed that some translation factors were dynamically methylated in response to the activity of MAT2A. These observations suggest that cells possess an mTOR-independent regulatory mechanism that tunes translation in response to the levels of SAM. Such a system may acclimate cells for survival when SAM synthesis is reduced, whereas it may support proliferation when SAM is sufficient.