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A new automated tool to quantify nucleoid distribution within mitochondrial networks
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AbstractMitochondrial DNA (mtDNA) maintenance is essential to sustain a functionally healthy population of mitochondria within cells. Proper mtDNA replication and distribution within mitochondrial networks are essential to maintain mitochondrial homeostasis. However, the fundamental basis of mtDNA segregation and distribution within mitochondrial networks is still unclear. To address these questions, we developed an algorithm, Mitomate tracker to unravel the global distribution of nucleoids within mitochondria. Using this tool, we decipher the semi-regular spacing of nucleoids across mitochondrial networks. Furthermore, we show that mitochondrial fission actively regulates mtDNA distribution by controlling the distribution of nucleoids within mitochondrial networks. Specifically, we found that primary cells bearing disease-associated mutations in the fission proteins DRP1 and MYH14 show altered nucleoid distribution, and acute enrichment of enlarged nucleoids near the nucleus. Further analysis suggests that the altered nucleoid distribution observed in the fission mutants is the result of both changes in network structure and nucleoid density. Thus, our study provides novel insights into the role of mitochondria fission in nucleoid distribution and the understanding of diseases caused by fission defects.
Springer Science and Business Media LLC
Title: A new automated tool to quantify nucleoid distribution within mitochondrial networks
Description:
AbstractMitochondrial DNA (mtDNA) maintenance is essential to sustain a functionally healthy population of mitochondria within cells.
Proper mtDNA replication and distribution within mitochondrial networks are essential to maintain mitochondrial homeostasis.
However, the fundamental basis of mtDNA segregation and distribution within mitochondrial networks is still unclear.
To address these questions, we developed an algorithm, Mitomate tracker to unravel the global distribution of nucleoids within mitochondria.
Using this tool, we decipher the semi-regular spacing of nucleoids across mitochondrial networks.
Furthermore, we show that mitochondrial fission actively regulates mtDNA distribution by controlling the distribution of nucleoids within mitochondrial networks.
Specifically, we found that primary cells bearing disease-associated mutations in the fission proteins DRP1 and MYH14 show altered nucleoid distribution, and acute enrichment of enlarged nucleoids near the nucleus.
Further analysis suggests that the altered nucleoid distribution observed in the fission mutants is the result of both changes in network structure and nucleoid density.
Thus, our study provides novel insights into the role of mitochondria fission in nucleoid distribution and the understanding of diseases caused by fission defects.
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