| Successful modification | The parasite was generated by the genetic modification |
| The mutant contains the following genetic modification(s) |
Gene disruption
|
| Reference (PubMed-PMID number) |
Reference 1 (PMID number) : 11349074
|
| MR4 number |
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| Parent parasite used to introduce the genetic modification |
| Rodent Malaria Parasite | P. berghei |
| Parent strain/line | P. berghei ANKA |
| Name parent line/clone |
P. berghei ANKA 2.34
|
| Other information parent line | P. berghei ANKA 2.34 is a cloned, gametocyte producer line of the ANKA strain (PubMed: PMID: 15137943). |
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| The mutant parasite was generated by |
| Name PI/Researcher | J.T. Dessens; R.E. Sinden |
| Name Group/Department | Department of Biolology |
| Name Institute | Imperial college of Science Technology and Medicine |
| City | London |
| Country | United Kingdom |
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| Name of the mutant parasite |
| RMgm number | RMgm-146 |
| Principal name | pbcht1-ko (clone 33 and 37) |
| Alternative name | |
| Standardized name | |
| Is the mutant parasite cloned after genetic modification | Yes |
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| Phenotype |
| Asexual blood stage | Not different from wild type |
| Gametocyte/Gamete | Not different from wild type |
| Fertilization and ookinete | Normal numbers of gametocytes, gametes, zygotes and mature ookinetes are formed. In Giemsa stained smears the morphology of mutant ookinetes is comparable to that of wild type ookinetes. Ookinetes have a reduced (30-90%) capacity to produce oocysts in A. stephensi mosquitoes(see phenotype 'Oocysts'). |
| Oocyst | When fed to A. stephensi mosquitoes, significant reductions in oocyst numbers of between 30 and 90% were obtained with the mutant parasites. The oocyst formed, produced normal numbers of sporozoites, that were infectious to the mammalian host. |
| Sporozoite | Not different from wild type |
| Liver stage | Not different from wild type |
| Additional remarks phenotype | Mutant/mutation
The mutant lacks expression of Chitinase (CHT1; Genbank accession number: AJ305256).
Protein (function)
CHT1, a secreted protein, is expressed in the ookinete stage and located in the micronemes. It contains putative proenzyme and chitin-binding domains. Chitinases are enzymes that hydrolize chitin, a (1-4)-β homopolymer of N-acetylglucosamine.
Phenotype
The phenotype analyses indicate a role during the transition of the ookinete into the oocyst stage (see also 'Additional information'). However, CHT1 is not essential for mosquito infectivity.
Additional information
Chitinase activity is thought to be critical for ookinetes to penetrate the chitin-containing peritophic matrix and midgut epithelial cells.
Feeding of in vitro cultured mature mutant ookinetes to A. stephensi resulted in the same reduction in oocyst formation as was found after feeding mutant gametocytes. In the ookinete feeds, the ookinetes invade the midgut cells before a perithrophic membrane is formed, suggesting that P. berghei chitinase is not involved in penetration of the perithrophic membrane.
The chitinase inhibitor allosamidin effectively abolished oocyst development of P. falciparum and P. gallinaceum. This inhibitor did not affect P. berghei infectivity in A. stephensi as measured by oocyst production, suggesting that allosamidin does not affect P. berghei CHT1.
CHT1 of P. falciparum is significantly different from P. berghei CHT1, in that the P. falciparum protein does not appear to be a pro-enzyme, nor does it appear to have a chitin-binding domain.
In P. falciparum a mutant has been generated with a disrupted gene encoding pfCHT1 (Y. Tsai et al., 2001, Infect. Immun. 69, 4048-54). This mutant had normal gametocytogenesis, exflagellation, and ookinete formation but was markedly impaired in its ability to form oocysts in Anopheles freeborni midguts.
Other mutants |
*RMgm-146
