Left-Right Axis Determination and Cardiac Development

左右轴测定和心脏发育

• 批准号: 6924652
• 负责人: ANN F RAMSDELL
• 金额: $ 29.1万
• 依托单位: UNIVERSITY OF SOUTH CAROLINA AT COLUMBIA
• 依托单位国家: 美国
• 财政年份: 2002
• 资助国家: 美国
• 起止时间: 2002-09-01 至 2008-07-31
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/6924652
• 关键词: Xenopus; Xenopus oocyte; biological signal transduction; biomarker; cell cell interaction; congenital cardiovascular disorder; gene expression; gene induction /repression; gene targeting; growth /development; growth factor receptors; heart cell; high throughput technology; histogenesis; inhibin; molecular cloning; morphology; nonmammalian vertebrate embryology; orientation; protein tyrosine kinase; transforming growth factors; transplantation

DESCRIPTION (provided by applicant): The majority of complex congenital heart defects occur in individuals who are also afflicted by laterality disease, reflecting the extreme susceptibility of the developing heart to disturbances in left-right (LR) patterning processes. The objective of this proposal is to identify inductive mechanisms that generate the LR body plan and to elucidate how cardiac cells use this positional "blueprint" to develop LR asymmetries. With focus on receptors for the transforming growth factor-Beta superfamily, we have found that two Activin-Like Kinases--ALK2 and ALK4--are both necessary and sufficient for LR development of the heart (and other organs) in embryos of the frog, Xenopus Iaevis. Taking advantage of the range of experimental manipulations that is uniquely possible in Xenopus, we will test the hypothesis that ALK2 and ALK4 modulate cardiac LR development by playing pivotal roles in LR axis determination. Using both biochemical and loss-of-function analyses, Aim 1 will identify cell-cell signals important for LR axis formation by defining ligands for the ALK pathways. Using classic transplantation and co-culture assays, Aim 2 will position ALK pathways in the context of cell-cell interactions already known to be important for LR patterning by determining whether ALKs relay positional signals to the midline. Because many of the molecules involved in midline specification and other LR relay interactions are not known, Aim 3 will fill in some of these gaps by identifying genes that function upstream, downstream, or within ALK pathways. This will be accomplished by performing a high throughput expression cloning screen in which new laterality genes already have been, and will continue to be, identified by the applicant. Using in vivo lineage labeling, Aim 4 will address how cardiac cells utilize LR patterning information by determining whether ALK signaling culminates in specific asymmetric cell contributions from the paired left and right heart fields to different segments of the "straight" heart tube. Together, our results will contribute new knowledge that is necessary to accelerate progress in the intersecting fields of embryonic heart formation and vertebrate LR development. The long-term significance of the work will be to identify genes and inductive processes that may result in congenital cardiac (and other) LR defects if affected by genetic or environmental perturbations.

描述（由申请人提供）：大多数复杂的先天性心脏缺陷发生在患有侧侧性疾病的个体中，反映了发育中的心脏对左右（LR）模式过程紊乱的极端易感性。本提案的目的是确定产生LR体计划的诱导机制，并阐明心肌细胞如何使用这种位置“蓝图”来发展LR不对称。重点关注转化生长因子- β超家族的受体，我们发现两种激活素样激酶——ALK2和ALK4——对于青蛙爪蟾胚胎心脏（和其他器官）的LR发育都是必要的和充分的。利用Xenopus独特的实验操作范围，我们将验证ALK2和ALK4通过在LR轴决定中发挥关键作用来调节心脏LR发展的假设。使用生化和功能丧失分析，Aim 1将通过定义ALK途径的配体来识别对LR轴形成重要的细胞-细胞信号。使用经典的移植和共培养试验，Aim 2将通过确定ALK是否将位置信号传递到中线，在已知对LR模式很重要的细胞-细胞相互作用背景下定位ALK通路。由于许多参与中线规范和其他LR中继相互作用的分子尚不清楚，Aim 3将通过识别在ALK途径上游、下游或内部起作用的基因来填补这些空白。这将通过执行高通量表达克隆筛选来完成，其中新的侧性基因已经被申请人识别，并将继续被申请人识别。利用体内谱系标记，Aim 4将通过确定ALK信号是否最终导致从配对的左、右心脏区到“直”心管的不同段的特定不对称细胞贡献，来解决心脏细胞如何利用LR模式信息。总之，我们的结果将为加速胚胎心脏形成和脊椎动物LR发育交叉领域的进展提供必要的新知识。这项工作的长期意义将是确定基因和诱导过程，如果受到遗传或环境扰动的影响，可能导致先天性心脏（和其他）LR缺陷。