Hox Genes & Lineage Infidelity
霍克斯基因
基本信息
- 批准号:10640862
- 负责人:
- 金额:$ 50.61万
- 依托单位:
- 依托单位国家:美国
- 项目类别:
- 财政年份:2019
- 资助国家:美国
- 起止时间:2019-09-01 至 2024-05-31
- 项目状态:已结题
- 来源:
- 关键词:ATAC-seqAbiesAdultAllelesAutomobile DrivingBindingBiological AssayBody partCell Differentiation processCellsChIP-seqChildChromatinCodeComplexConfusionDataData SetDefectDevelopmentDifferentiated GeneDiseaseDistalDrosophila genusDuct (organ) structureEpigenetic ProcessEpitopesFrameshift MutationGene ExpressionGene MutationGenesGeneticHOX proteinHeadHenle&aposs loopHistonesHomeobox GenesImmunofluorescence ImmunologicIndividualInjury to KidneyIschemiaKidneyLectinLegLysineMammalsMediatingMethylationModelingMusMutateMutationNatural regenerationNephronsOrganOrganismPRC1 ProteinPaperPathway interactionsPhenotypePolycombPreventionProteinsRegulator GenesRenal tubule structureReperfusion TherapyRepressionResearchRoleScientistSeriesSpecific qualifier valueStainsTestingTissuesUbiquitinationUncertaintyWorkcell typecombinatorialderepressionexperimental studygene functiongene repressionimaginal discinsightmutantnovelparalogous genepreservationprotein complexrepairedsingle-cell RNA sequencingtranscription factortranscriptome sequencing
项目摘要
Abstract
Hox gene mutations in simpler organisms often resulting in dramatic homeotic transformations of one
body part into another. They encode transcription factors that can initiate genetic cascades that drive the
developmental destinies of segments. In mammals there are 39 Hox genes, in four clusters, divided into 13
functionally related paralog groups. It is necessary to mutate multiple Hox genes from multiple paralog groups
to overcome redundancies and reveal previously hidden shared functions. To this end we have made mice
with frameshift mutations in sets of adjacent Hox genes. By interbreeding we can dial down Hox function for
multiple paralog groups while maintaining sufficient Hox11 expression to have a developing kidney to study.
Mice with simultaneous frameshift mutation of twelve closely related Hox9,10,11 alleles show a very
unexpected kidney phenotype. The cells of the mutant nephrons often show mixed identities, with co-
expression of markers of more than one segment cell type. This was examined with an extensive battery of
segment specific markers. Providing further confirmation, Hox mutation in Drosophila can also lead to de-
repression of many genes normally expressed in other lineages, very similar to what we see in mice.
In specific aim 1 we propose to further study the apparently confused, mixed identity character of the
multi-Hox mutants using single cell RNA-seq and single cell ATAC-seq, to define the limits of the crossing of
lineage boundaries and to search for underlying mechanisms. How many different cell type markers can be
expressed by an individual cell? Do open/closed chromatin configurations in mutants reveal even more
epigenetic plasticity than seen by RNA-seq? Are there perturbations in pathways that suggest mechanisms?
In specific aim 2 we test the hypothesis that the observed mixed cell identity mutant phenotype is the
result of disrupted Polycomb Repressive Complex (PRC) function. Cell type specific transcription factors
initially establish repressed gene expression states, and then PRC complexes recognize and maintain their
repression. Work in Drosophila has shown that Hox proteins and PRC proteins can co-bind to drive repression
of inappropriate cell type genes. In this aim we carry out a series of Chip-seq experiments to compare wild
type/mutant distributions of PRC1 (H2Aub1), PRC2 (H3K27me3), active (H3K4me3), Hoxa11 and Hoxd11
(using our epitope tagged mice), as well as Ezh2 and Ring1B PRC component proteins.
In specific aim 3 we propose to test the hypothesis that Hox genes also function to reduce cell type
plasticity in the adult. Hox genes generally continue to be expressed in the adult. The function for this has
remained uncertain, although it has been proposed that it serves to maintain expression of the appropriate
differentiation genes. We propose that it also serves to maintain repression of inappropriate differentiation
genes. We propose to carry out single cell RNA-seq experiments on ischemia reperfusion wild type and Hox
mutant injured kidneys, where cells normally de-differentiate and then re-differentiate, to test his hypothesis.
摘要
项目成果
期刊论文数量(0)
专著数量(0)
科研奖励数量(0)
会议论文数量(0)
专利数量(0)
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Joo-Seop Park其他文献
Joo-Seop Park的其他文献
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{{ truncateString('Joo-Seop Park', 18)}}的其他基金
Hedgehog gene regulatory networks in the mammalian kidney
哺乳动物肾脏中的刺猬基因调控网络
- 批准号:
10544169 - 财政年份:2022
- 资助金额:
$ 50.61万 - 项目类别:
Hedgehog gene regulatory networks in the mammalian kidney
哺乳动物肾脏中的刺猬基因调控网络
- 批准号:
10344254 - 财政年份:2022
- 资助金额:
$ 50.61万 - 项目类别:
Gene regulatory networks in the proximal tubules of the mammalian kidney
哺乳动物肾脏近端小管的基因调控网络
- 批准号:
10031038 - 财政年份:2020
- 资助金额:
$ 50.61万 - 项目类别:
Gene regulatory networks in the proximal tubules of the mammalian kidney
哺乳动物肾脏近端小管的基因调控网络
- 批准号:
10187563 - 财政年份:2020
- 资助金额:
$ 50.61万 - 项目类别:
Retinoic acid gene regulatory networks in the mammalian kidney
哺乳动物肾脏中的视黄酸基因调控网络
- 批准号:
9898363 - 财政年份:2019
- 资助金额:
$ 50.61万 - 项目类别:
Retinoic acid gene regulatory networks in the mammalian kidney
哺乳动物肾脏中的视黄酸基因调控网络
- 批准号:
10337216 - 财政年份:2019
- 资助金额:
$ 50.61万 - 项目类别:
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