Medical Biology - Theses

Permanent URI for this collection

http://hdl.handle.net/11343/239

Filters

2022 1
1
Reset filters

Settings
Statistics
Citations
Author: Krol, Jelte Martinus Maria × End date: 2023 × Start date: 2020 × Subject: Malaria × Subject: Plasmodium ×

Search Results

Now showing 1 - 1 of 1
  • Item
    Thumbnail Image
    Identifying and Characterising Exported Hepatic Effector Proteins of the Human Malaria Parasite Plasmodium falciparum
    Krol, Jelte Martinus Maria ( 2022)
    The parasitic disease malaria is caused by symptomatic infection of Plasmodium parasites during their infection in erythrocytes. Plasmodium falciparum, the most lethal parasite that infects humans, must first undergo replication during the asymptomatic liver stage, which makes it a primary target for prophylactic intervention. Our current understanding of P. falciparum liver stage biology is limited, particularly around the parasite’s ability to subvert host innate defences and exploit host nutrients. This is due to the limited models for liver stage research as P. falciparum replicates in the hepatocyte for 7 days forming tens of thousands of merozoites in an enclosed parasitophorous vacuole. Merozoites in turn infect erythrocytes upon liver stage egress and subsequent release into the blood stream. By infecting an erythrocyte, the parasite forms a parasitophorous vacuole and exports proteins across this vacuole membrane into the host, leading to molecular changes causing malaria-associated pathology. Many parasitic proteins are targeted for export by a pentameric amino-acid motif known as the PEXEL (RxLxE/D/Q), that is proteolytically cleaved in the ER by the aspartyl protease plasmepsin V. Matured effector proteins, as well as PEXEL-negative exported proteins, are translocated into the host-cytoplasm by the PTEX complex. The process of protein export has been widely studied during blood stage infection, but little is known about this process during liver stage. Important questions are whether the export pathway is active and important during the liver stage of the parasite life cycle and whether effector proteins can be identified. In this PhD. we are aiming to address these questions by attempting to identify and characterise novel liver stage exported proteins using two approaches. First, an agnostic approach involving proximity ligation proteomics has been hypothesised to identify liver-stage proteins in subcellular compartments of the parasite and host cell. Second, PEXEL-searching has identified 20 effector candidates of which some have been visualised utilising epitope tagged parasites and polyclonal antibodies. Some effectors have been functionally characterised using rapamycin-mediated conditional gene excision to disrupt expression of respective genes during the P. falciparum life cycle. In vitro sporozoite invasion and traversal assays as well as in vivo liver stage experiments utilising chimeric mice with engrafted human hepatocytes were used to demonstrate the role of these proteins during liver stage. Future identification of novel P. falciparum liver stage exported proteins may provide new drug and vaccine targets for preventive therapeutics targeting the pre-erythrocytic stage of infection by malaria parasites that infect humans.