Tbx18-Cre基因敲入小鼠的繁殖、鉴定及其应用

为了探讨Tbx18-Cre基因敲入小鼠(Tbx18:Cre knock-in Mus musculus)的繁殖、鉴定及Tbx18基因敲除小鼠和遗传示踪小鼠模型的应用,将Tbx18-Cre基因敲入杂合子小鼠进行繁殖,应用PCR法鉴定其子代基因型。将子代雌雄杂合子小鼠互交,应用H.E染色观察Tbx18基因敲除胚鼠心的形态学变化。将杂合子小鼠与RosaEYFP报告小鼠交配,应用心冰冻切片技术观察Tbx18:Cre/Rosa26REYFP双转基因遗传示踪胚鼠心内Tbx18阳性心外膜祖细胞发育命运。结果表明,用于繁殖、基因敲除研究及基因遗传示踪的子代基因型均符合孟德尔遗传规律。同时心H.E染色和心冰冻切片发现,Tbx18敲除小鼠心窦房结发育存在缺陷,而Tbx18阳性心外膜祖细胞是心发育重要的祖细胞来源。研究结果揭示,Tbx18-Cre基因敲除小鼠是研究先天性心脏病发病机制的理想模式动物,Tbx18阳性心外膜祖细胞可能是心脏病患者心脏修复和再生潜在的种子细胞。     

Tbx18对小鼠心脏冠状血管及室壁结构发育的影响

利用Tbx18谱系示踪小鼠模型及Tbx18条件性基因敲除小鼠模型,探讨转录因子Tbx18对小鼠心血管结构发育的影响.实验建立Tbx18-Cre/Rosa26R-EYFP和Tbx18-Cre/Rosa26R-Lac Z两种基因敲入谱系示踪小鼠模型和Tbx18:Cre/Cre基因敲除小鼠模型;通过免疫荧光及X-gal染色技术,示踪Tbx18在心血管系统结构形成中的命运;通过小鼠心脏整体血管免疫组化及切片HE染色、免疫组化、免疫荧光技术,比较Tbx18:Cre/Cre基因敲除小鼠与野生型对照小鼠心脏室壁结构及冠状血管结构发育情况.示踪结果提示,Tbx18参与小鼠冠状血管及室间隔结构的形成,并与冠脉平滑肌细胞共表达;对Tbx18基因敲除小鼠及野生型小鼠的心脏结构比较提示,Tbx18基因敲除后,仍能形成形态正常的冠状血管系统,小鼠心室肌及室间隔厚度较野生型无明显差异.结果表明,Tbx18参与小鼠心脏血管平滑肌及室间隔结构的形成,但其在小鼠心脏腔室结构及冠状血管结构形成过程中不是必需的.     

谱系示踪技术揭示Tbx18+肾脏祖细胞分化为脂肪细胞

转录因子Tbx18在泌尿系发育中发挥重要作用。利用遗传谱系示踪模型，揭示了Tbx18+肾祖细胞具有向多种肾系细胞分化的潜能。但尚无文献报道其是否具有向脂肪细胞分化的潜能。本研究通过对Tbx18Cre/Rosa26LacZ双杂合小鼠泌尿系组织进行整体X-gal染色发现，肾包膜、输尿管及肾周脂肪组织能特异性表达β-gal蛋白，说明肾包膜、输尿管及肾周脂肪组织可能来源于Tbx18+祖细胞。对Tbx18Cre/Rosa26EYFP双杂合小鼠泌尿系组织进行免疫荧光染色，发现部分脂滴相关蛋白+（perilipin）脂肪细胞能表达标记蛋白EYFP，说明部分泌尿系脂肪细胞来源于Tbx18+祖细胞。本研究揭示了Tbx18+祖细胞具有分化为脂肪细胞的潜能，进一步证实了Tbx18+肾祖细胞的多分化潜能。结合本研究结果，若进一步研究肾损伤时，来源于Tbx18+祖细胞的泌尿系脂肪细胞是否进一步增多，将会为肾损伤的再生修复提供一些思路和启发。     

基因谱系示踪揭示Tbx18+祖细胞的多分化潜能

为探讨Tbx18+祖细胞在小鼠生长发育过程中的多分化潜能及分化的组织类型,本工作建立了Tbx18：Cre/Rosa26RLacZ谱系示踪小鼠.该示踪小鼠基于Cre/LoxP系统,能够准确及有效地示踪Tbx18+祖细胞的分化命运,通过整体胚胎及组织X-gal染色,检测分析报告基因LacZ在其中的表达情况.结果显示,在Tbx18：Cre/Rosa26RLacZ双杂合小鼠胚胎发育早期,报告基因LacZ主要在脊柱、四肢及心外膜表达|而在胚胎发育晚期则分别表达于皮肤、毛囊、肾脏、输尿管、膀胱、睾丸、输精管、椎间盘、肋软骨、心耳、心肌、冠状动脉.结果阐明,Tbx18+祖细胞在小鼠生长发育过程中具有强大的多器官及组织分化潜能,包括分化形成表皮系统,泌尿生殖系统,骨骼系统,心血管系统,并在其生长发育中发挥重要作用.     

谱系示踪技术揭示Tbx18~+肾祖细胞分化为脂肪细胞的潜能

转录因子Tbx18在泌尿系发育中发挥重要作用。利用遗传谱系示踪模型,揭示了Tbx18~+肾祖细胞具有向多种肾系细胞分化的潜能。但尚无文献报道其是否具有向脂肪细胞分化的潜能。本研究通过对Tbx18Cre/Rosa26~(LacZ)双杂合小鼠泌尿系组织进行整体X-gal染色发现,肾包膜、输尿管及肾周脂肪组织能特异性表达β-gal蛋白,说明肾包膜、输尿管及肾周脂肪组织可能来源于Tbx18+祖细胞。对Tbx18Cre/Rosa26~(EYFP)双杂合小鼠泌尿系组织进行免疫荧光染色,发现部分脂滴相关蛋白~+(perilipin)脂肪细胞能表达标记蛋白EYFP,说明部分泌尿系脂肪细胞来源于Tbx18~+祖细胞。本研究揭示了Tbx18~+祖细胞具有分化为脂肪细胞的潜能,进一步证实了Tbx18~+肾祖细胞的多分化潜能。结合本研究结果,若进一步研究肾损伤时,来源于Tbx18~+祖细胞的泌尿系脂肪细胞是否进一步增多,将会为肾损伤的再生修复提供一些思路和启发。     

Tbx18通过下调EMT信号分子参与调控心脏发育

转录因子Tbx18(Tbx18)在小鼠胚胎心外膜上皮细胞表达并调控心外膜上皮细胞向心系细胞分化.上皮间充质转化(EMT)过程是器官发育和形成的重要机制.为阐述Tbx18通过调控下游EMT关键信号分子参与心外膜上皮细胞分化和心脏发育,本研究运用Tbx18-Cre/Rosa26R-EYFP双杂合基因敲入小鼠和免疫荧光共聚焦,证实Tbx18+心系细胞和EMT关键信号分子Snail1、Smad、Slug、Twist在发育后期胚鼠心外膜和心外膜下间充质发生共聚焦.同时还发现,Tbx18在胚鼠不同发育阶段的表达模式和Tbx18+心系细胞内上述EMT关键信号分子的表达模式相似.Tbx18和EMT关键信号分子在发育心脏存在相似的时空表达模式,因此,它们之间可能存在相互调控作用.运用Tbx18突变技术揭示了Tbx18突变型胚鼠心脏EMT关键信号分子表达水平均较野生型显著下调,直接证实了上述4个EMT信号分子是Tbx18的可能靶点.理解Tbx18参与心脏发育的下游靶点有助于改善成年心脏损伤后的再生修复.     

基因谱系示踪揭示小鼠Tbx18+肾脏间质祖细胞分化为输尿管平滑肌

本文旨在研究Tbx18+肾脏间质祖细胞分化为输尿管平滑肌细胞的命运及转录因子Tbx18在小鼠输尿管平滑肌发育形成中起到的作用．实验建立Tbx18:Cre/R26REYFP和Tbx18:Cre/R26RLacZ两种谱系示踪系统和Tbx18:Cre/Cre 敲除模型．该示踪模型通过cre重组酶的表达能有效地示踪Tbx18+肾脏间质祖细胞在泌尿系统的发育命运．通过免疫荧光染色和X-gal染色,同时发现Tbx18+肾脏间质祖细胞可分化为输尿管平滑肌细胞,但不分化为输尿管移行上皮细胞．在Tbx18:Cre/Cre基因突变模型中,泌尿系统出现明显的肾积水和输尿管积水,肾盏、肾盂扩张,输尿管明显缩短和扩张．实验结果揭示,Tbx18+ 肾脏间质祖细胞可以分化为输尿管平滑肌细胞,且转录因子Tbx18在哺乳动物输尿管平滑肌的发育中起到重要的作用．     

利用CRISPR/Cas9技术构建CreERT2定点敲入Isl1基因小鼠模型及分析

心肌祖细胞增殖和分化是心脏损伤后修复再生的基础,而Isl1被认为是心肌祖细胞的特异性标志。为了研究以及示踪Isl1+心肌祖细胞及其分化后代,该文尝试利用成簇规律间隔短回文重复序列CRISPR/Cas9系统,将Cre ERT2定点插入到小鼠Isl1内源基因启动子之后,建立了Cre ERT2基因敲入小鼠模型。通过与Rosa26-lox P-neo-lox P-lac Z小鼠(Rosa26-lac Z+)交配,获得Isl1-Cre ERT(KI)/Rosa26-lac Z+双杂合小鼠。经过基因型鉴定、组织表达谱测定和X-gal染色、冰冻切片和石蜡切片等方法,确认基因敲入小鼠的Cre ERT2表达在成年小鼠心脏窦房结、心脏神经节、主动脉弓和肺动脉根部,与文献报道的Isl1表达部位相同。该研究建立的模型可为研究心肌祖细胞的增殖和谱系示踪提供重要的模型。     

Tbx18+心外膜祖细胞参与成年小鼠部分心脏组织形成

转录因子Tbx18在胚胎心脏发育过程中起重要调控作用,是心外膜祖细胞标记之一|故以Tbx18为标记的阳性祖细胞群被称为：Tbx18+心外膜祖细胞(epicardial progenitor cells, EPCs)。小鼠胚胎、新生和成年期心脏组织细胞的特性区别较大,成年小鼠的心脏属于终末分化组织。但是,Tbx18+EPCs对成年小鼠心脏组织的贡献大小尚存争议。本研究拟定量分析Tbx18+EPCs对成年小鼠心脏组织的贡献大小。采用整体和组织切片X-gal染色检测成年心脏组织LacZ的表达|荧光激活细胞分选法(fluorescence activated cell sorting,FACS)分离成年Tbx18Cre/R26EYFP小鼠心脏组织EYFP+细胞。结果显示,在Tbx18+EPCs遗传谱系示踪小鼠,报告基因LacZ和EYFP在成年小鼠心脏的心室、心房、冠状动脉、室间隔等处表达|成年Tbx18Cre/R26EYFP小鼠心脏组织细胞用FACS分离,分选的EYFP+细胞比例平均约为33.94%。由此可见,成年小鼠心脏的心室、心房、冠状动脉、室间隔等心脏组织均可来源于Tbx18+EPCs|约1/3成年小鼠心脏组织细胞来源于Tbx18+EPCs。故Tbx18+EPCs参与成年小鼠心脏组织的部分形成。     

遗传谱系示踪技术揭示小鼠胚胎前体心外膜向心外膜转化过程

心外膜的形成是胚胎心脏发育的关键生理过程之一。利用遗传谱系示踪技术示踪观察前体心外膜向心外膜细胞转化过程,具有重要的科学研究价值。本研究拟利用Tbx18+前体/心外膜祖细胞遗传谱系示踪模型,揭示胚胎心外膜的起源及前体心外膜向心外膜转化的过程。利用整胚和切片原位杂交技术揭示,Tbx18 mRNA特异性表达于胚龄（E）9.5 d小鼠胚胎前体心外膜;故Tbx18是前体心外膜的特异性标记基因。利用整胚X-Gal染色,揭示报告基因Lacz在E9.5 d遗传谱系示踪模型鼠胚前体心外膜中大量表达,此时报告基因从前体心外膜逐渐迁移并开始少量表达于心外膜。Lacz在E10～E10.5 d双杂合鼠胚前体心外膜中表达逐渐减少,而在心外膜组织中逐渐增多;在E11.5 d,报告基因在前体心外膜中表达基本消失,而在心外膜组织中大量表达。切片进行X-Gal染色也揭示,报告基因Lacz定位于早期胚胎前体心外膜及心外膜。免疫荧光染色证实,早期胚胎心外膜细胞呈现未分化的祖细胞状态。通过报告基因的表达变化模式揭示,胚胎心外膜的形成经历了启动、转化、完成3个阶段;E9.5～11.5 d左右这个时间段发生的前体心外膜向心外膜转化,可能是心外膜形成的主要来源和形式。     

Reassessment of Isl1 and Nkx2-5 cardiac fate maps using a Gata4-based reporter of Cre activity

Isl1 and Nkx2-5-expressing cardiovascular progenitors play pivotal roles in cardiogenesis. Previously reported Cre-based fate-mapping studies showed that Isl1 progenitors contribute predominantly to the derivatives of the second heart field, and Nkx2-5 progenitors contributed mainly to the cardiomyocyte lineage. However, partial recombination of Cre reporter genes can complicate interpretation of Cre fate-mapping experiments. We found that a Gata4-based Cre-activated reporter was recombined by Isl1^Cre and Nkx2-5^Cre in a substantially broader domain than previously reported using standard Cre-activated reporters. The expanded Isl1 and Nkx2-5 cardiac fate maps were remarkably similar, and included extensive contributions to cardiomyocyte, endocardial, and smooth muscle lineages in all four cardiac chambers. These data indicate that Isl1 is expressed in progenitors of both primary and secondary heart fields, and that Nkx2-5 is expressed in progenitors of cardiac endothelium and smooth muscle, in addition to cardiomyocytes. These results have important implications for our understanding of cardiac lineage diversification in vivo, and for the interpretation of Cre-based fate maps.     

Progenitors of skeletal muscle satellite cells express the muscle determination gene, MyoD

Satellite cells are tissue-specific stem cells responsible for skeletal muscle growth and regeneration. Although satellite cells were identified almost 50 years ago, the identity of progenitor populations from which they derive remains controversial. We developed MyoD^iCre knockin mice, and used Cre/lox lineage analysis to determine whether satellite cell progenitors express MyoD, a marker of myogenic commitment. Recombination status of satellite cells was determined by confocal microscopy of isolated muscle fibers and by electron microscopic observation of muscle tissue fixed immediately following isolation, using R26R-EYFP and R26R (β-gal) reporter mice, respectively. We show that essentially all adult satellite cells associated with limb and body wall musculature, as well as the diaphragm and extraocular muscles, originate from MyoD+ progenitors. Neonatal satellite cells were Cre-recombined, but only a small minority exhibited ongoing Cre expression, indicating that most satellite cells had expressed MyoD prenatally. We also show that satellite cell development in MyoD-null mice is not due to functional compensation by MyoD non-expressing lineages. The results suggest that satellite cells are derived from committed myogenic progenitors, irrespective of the anatomical location, embryological origin, or physiological properties of associated musculature.     

Nkx2-5- and Isl1-expressing cardiac progenitors contribute to proepicardium

Correct delineation of the hierarchy of cardiac progenitors is a key step to understanding heart development, and will pave the way for future use of cardiac progenitors in the treatment of heart disease. Multipotent Nkx2-5 and Isl1 cardiac progenitors contribute to cardiomyocyte, smooth muscle, and endothelial lineages, which constitute the major lineages of the heart. Recently, progenitors located within the proepicardium and epicardium were reported to differentiate into cardiomyocytes, as well as smooth muscle and endothelial cells. However, the relationship of these proepicardial progenitors to the previously described Nkx2-5 and Isl1 cardiac progenitors is incompletely understood. To address this question, we performed in vivo Cre-loxP-based lineage tracing. Both Nkx2-5- and Isl1-expressing progenitors contributed to the proepicardium and expressed Wt1 and Tbx18, markers of proepicardial progenitor cells. Interestingly, Nkx2-5 knockout resulted in abnormal proepicardial development and decreased expression of Wt1, suggesting a functional role for Nkx2-5 in proepicardium formation. Taken together, these results suggest that Nkx2-5 and/or Isl1 cardiac progenitors contribute to proepicardium during heart development.     

The contribution of the Tie2+ lineage to primitive and definitive hematopoietic cells

The regulatory elements of the Tie2/Tek promoter are commonly used in mouse models to direct transgene expression to endothelial cells. Tunica intima endothelial kinase 2 (Tie2) is also expressed in hematopoietic cells, although this has not been fully characterized. We determine the lineages of adult hematopoietic cells derived from Tie2‐expressing populations using Tie2‐Cre;Rosa26R‐EYFP mice. In Tie2‐Cre;Rosa26R‐EYFP mice, analysis of bone marrow cells showed Cre‐mediated recombination in 85% of the population. In adult bone marrow and spleen, we analyzed subclasses of early hematopoietic progenitors, T cells, monocytes, granulocytes, and B cells. We found that ～ 84% of each lineage was EYFP⁺, and nearly all cells that come from Tie2‐expressing lineages are CD45⁺, confirming widespread contribution to definitive hematopoietic cells. In addition, more than 82% of blood cells within the embryonic yolk sac were of Tie2⁺ origin. Our findings of high levels of Tie2‐Cre recombination in the hematopoietic lineage have implications for the use of the Tie2‐Cre mouse as a lineage‐restricted driver strain. genesis 48:563–567, 2010. © 2010 Wiley‐Liss, Inc.