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Gary Ward, PhD
Professor
Research Interests
Toxoplasma
gondii is a protozoan parasite that causes severe congenital disease
in newborn infants, and life-threatening disease in people whose immune
systems have been weakened by immunosuppressants, age or AIDS. The tissue
destruction associated with toxoplasmosis is in large part due to repeated
cycles of host cell invasion, parasite multiplication and host cell lysis.
A better understanding of the mechanisms of host cell invasion by T.
gondii is therefore important to the development of new approaches
to the treatment of the disease it causes. T. gondii is also a powerful
model for studying invasive mechanisms in related, but less experimentally
tractable, protozoan parasites within the Phylum Apicomplexa, including
Plasmodium (the causative agent of malaria) and Cryptosporidium.
Our research is directed towards identifying T. gondii proteins
that play a role in host cell invasion and determining what these proteins
do. We have studied in detail the function of one specific protein, TgAMA1,
and we have developed more general, small-molecule-based approaches to
identifying previously uncharacterized invasion-related proteins.
TgAMA1. Using a combination of photoaffinity labeling (Gilk
et al, 2006) and targeted monoclonal antibody screening (Ward and
Carey, 1999), we identified and characterized several novel secreted and
surface proteins of T. gondii (Carey et al, 2000, 2004;
Gaskins et al, 2004; Gilk et al, 2006). One of these proteins,
TgAMA1 (Donahue et al, 2000), was of particular interest to us.
It is a member of a family of proteins that we now know is widely conserved
in apicomplexan parasites. Considerable indirect evidence had accumulated
suggesting a role for Plasmodium AMA1 in invasion, and Plasmodium
AMA1 was - and remains - a leading malaria vaccine candidate. Nonetheless,
despite almost two decades of intense interest in AMA1 family proteins,
little was known about their function. This was in part because AMA1 is
an essential gene; attempts to disrupt AMA1 for functional studies had
been uniformly unsuccessful.
Using a recently developed system for conditional gene expression in T.
gondii, we generated a parasite line in which the expression of TgAMA1
could be experimentally controlled (Mital et al, 2005). A decrease
in TgAMA1 expression in these conditional knockout parasites causes a
dramatic decrease in their invasiveness, providing direct evidence that
TgAMA1 plays a critical role in invasion. Further phenotypic analysis
of the mutants suggested that attachment of T. gondii to host cells occurs
in two distinct stages, the second of which requires TgAMA1 and is involved
in regulating secretion from the rhoptries, apical secretory organelles
that function in invasion (Mital et al, 2005). TgAMA1 also appears
to play an important role in forming the junction between the parasite
and the host cell, through which the parasite physically pulls itself
during invasion (Alexander et al, 2005).
TgAMA1 is stored in apical secretory organelles known as the micronemes,
and released onto the parasite surface during invasion. There, it is proteolytically
cleaved within its transmembrane domain and "shed" from the
parasite. The shedding of microneme proteins during invasion is a common
phenomenon in apicomplexan parasites, but its functional significance
remains unknown. The intramembrane cleavage site of TgAMA1 was recently
determined; we are using this information, together with our TgAMA1 conditional
knockout parasites, to determine the functional consequences of mutations
in the transmembrane domain that disrupt TgAMA1 cleavage and shedding.
Small-molecule-based approaches. In contrast to reverse
genetic approaches, such as the one just described for TgAMA1, forward
genetic approaches have the advantage of being assumption-free, i.e.,
they require no preconceived ideas about what gene products are important.
Unfortunately, standard forward genetic approaches to studying invasion
in haploid, obligate intracellular parasites such as T. gondii
are problematic, since the disruption of any gene essential for invasion
will likely be lethal. The generation of conditional knockouts/knockdowns
offers one potential way around this problem; we have developed an alternative
approach, in which large collections of structurally diverse small molecules
are screened for compounds that affect invasion, and then used as probes
to identify the relevant invasion-associated gene products.
In one such screen, 12,160 small molecules were assayed, resulting in
the identification of 24 novel, non-cytotoxic inhibitors of T. gondii
invasion (Carey et al, 2004). Unexpectedly, the screen also identified
six small molecules that dramatically enhance invasion. Secondary
assays demonstrated that the different inhibitors/enhancers perturb different
aspects of invasion, including gliding motility, cytoskeletal rearrangement,
and microneme secretion. Some have similar effects on other apicomplexan
parasites, suggesting that they target conserved component(s) of the apicomplexan
invasion machinery.
The small molecules we have identified in this and other screens represent
a powerful new set of tools for studying invasion, and we are currently
exploring specific hypotheses regarding their mechanisms of action. We
are using biochemical, synthetic and molecular genetic techniques to identify
their target(s) (e.g. Haraldsen et al, 2007) and to determine
the roles that these target molecules play in the process of invasion.
Target identification is typically the most difficult aspect of a small-molecule
approach (Ward et al, 2002), but is facilitated in our case by
the recently released sequence of the T. gondii genome, the molecular
genetic tools available in T. gondii and the extent to which we
are integrating biological experiments and synthetic chemistry (in collaboration
with Dr. Nick Westwood's group at the University of St. Andrews). In addition
to providing new probes for studying the mechanisms of host cell invasion,
this work has clear and exciting drug development implications for T.
gondii, and perhaps for other apicomplexan parasites as well.