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Synergistic Regulation of Border Cell Migration by Singed and Arp2/3 Complex in Drosophila: Insights into F-Actin Dynamics

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dc.contributor.advisor PANANGHAT, GAYATHRI
dc.contributor.advisor Majumder, Pralay
dc.contributor.author PEGU, NETRA
dc.date.accessioned 2024-05-16T07:07:27Z
dc.date.available 2024-05-16T07:07:27Z
dc.date.issued 2024-05
dc.identifier.citation 40 en_US
dc.identifier.uri http://dr.iiserpune.ac.in:8080/xmlui/handle/123456789/8796
dc.description.abstract Stages 8, 9, and 10 of Drosophila oogenesis are critical for border cell (BC) migration. During stage 8, migration initiation occurs, while stage 9 sees BCs traversing nurse cells toward the oocyte. By stage 10, BCs reach the oocyte, necessitating close contact. In collective cell migration (CCM), the leading cells in the cohort generate forward protrusions, and lagging cells make backward retractions in a harmonized and concerted manner. Effectively, the actin cytoskeleton stands as the leading driver of protrusion formation and retractions. Using Drosophila melanogaster as a model, we study collective cell migration (CCM) in border cells (BCs). Singed (the vertebrate homolog of fascin) and the Arp2/3 complex genetically interact to regulate F-actin architecture in BCs. Depletion of both hindered migrations, leading to a substantial cell migration defect. Both collaborate to regulate F-actin density in border cell clusters. The consequence of F-actin alteration is manifested upon cluster shape and area as clusters become large and rounded. As the BC cluster’s shape depends on mechanical and physiological behavior of the individual border cell, we can predict a relationship between shape increase and border cell number. Our experiment focuses on three signaling pathways governing migration: a global steroid-hormone signal coordinating migration timing, a localized cytokine signal activating the Jak-Stat pathway for migration induction, and a growth factor guiding cells to their destination. We have made an experimental setup to observe each of the individual cells of the cluster and count their number through fixed imaging for both control and double knockdown. Furthermore, we are trying to find the correlation of stat92E and slbo with singed and arp2 during border cell migrations through genetic interaction studies. en_US
dc.language.iso en en_US
dc.subject Border cell en_US
dc.subject Collective cell migration en_US
dc.subject Singed en_US
dc.subject Arp2/3 en_US
dc.title Synergistic Regulation of Border Cell Migration by Singed and Arp2/3 Complex in Drosophila: Insights into F-Actin Dynamics en_US
dc.type Thesis en_US
dc.description.embargo Two Years en_US
dc.type.degree BS-MS en_US
dc.contributor.department Dept. of Biology en_US
dc.contributor.registration 20191168 en_US


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  • MS THESES [1705]
    Thesis submitted to IISER Pune in partial fulfilment of the requirements for the BS-MS Dual Degree Programme/MSc. Programme/MS-Exit Programme

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