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Susan R. Ross
Professor, Dept of
Microbiology
Microbiology,
Virology and Parasitology Program
Address
313 Biomedical Rsch Bldg (BRB) II/III (office)
324 Biomedical Rsch Bldg (BRB) II/III (lab)
421 Curie Boulevard
Philadelphia, PA 19104
Office tel.: 215 898-9764
Lab tel.: 215 898-2986
Fax: 215 573-2028
E-mail: rosss@mail.med.upenn.edu
Link(s)
Dr.
Ross's Microbiology Faculty Page
Education
University of Pennsylvania: BA (Biochemistry), 1975.
Princeton University: PhD (Biochemical Sciences), 1979.
University of California, San Francisco: Postdoctoral Research (Hormone regulation
of transcription) 1979-1982.
The Wistar Institute: Postdoctoral Research (Mouse genetics/transgenic mice) 1982-1983.
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Research
Interests
- genetic approaches to the study of host-virus
interactions.
Key words: retrovirus, transferrin receptor,
superantigen, toll receptor, mouse genetics.
Search PubMed for articles
Description
of Research
All animals show differential susceptibility
to infection with viruses. We use mouse mammary tumor virus
(MMTV), an endemic mouse retrovirus, to understand virus/host
interactions, since the genetics of susceptibility is easily
studied with naturally-occurring pathogens in inbred and genetically-manipulated
mice. Infectious MMTV is passed from mothers to offspring
through milk and first spreads in lymphoid cells before infecting
mammary epithelial cells. MMTV causes breast cancer when the
viral genome inserts next to cellular oncogenes, thereby activating
their expression. Our studies focus on understanding the mechanisms
that determine susceptibility to MMTV infection and virus-induced
mammary tumors.
One area of investigation in the lab is how
retroviruses infect their initial targets in vivo, since most
require activated cells as their targets for infection. We
showed that MMTV activates dendritic and B cells via toll-like
receptor 4 (TLR4), a component of the innate immune system;
we also demonstrated that dendritic cells are the initial
targets of infection in vivo. The dendritic and B cells of
mice with tlr4 mutations show diminished activation by MMTV.
MMTV interacts with TLR4 through binding of its envelope protein;
more recently, we have discovered that MMTV signals through
and binds to another toll-like receptor, TLR2. We are currently
focused on determining how dendritic cell infection and TLR
signaling affects host immune responses to MMTV.
Another gene which we recently discovered is
involved in the control of MMTV infection is apobec3. The
genomes of all mammals encode apobec3 genes which play a role
in intrinsic cellular immunity to a number of viruses, including
human immunodeficiency virus type 1. APOBEC3 proteins are
packaged into virions and inhibit retroviral replication in
newly infected cells, at least in part by deaminating cytosine
on the negative strand DNA intermediates. We found that mouse
APOBEC3 protein is packaged into MMTV particles in vitro and
dramatically reduces viral titers. Most importantly, APOBEC3
knockout mice are more susceptible to MMTV infection compared
to their wild type littermates. These findings indicate that
the APOBEC3 provides protection to mice against MMTV infection
and represent the first demonstration that it functions during
retroviral infection in vivo. Whether the accelerated infection
and spread of MMTV in mA3 -/- mice affects its ability to
cause breast cancer is currently under investigation.
We also identified another genetic locus in
C3H/HeN mice that confers dominant susceptibility to MMTV
infection in backcrosses with B10.BR mice, which are relatively
resistant to milk-borne infection and mammary tumorigenesis.
We mapped the locus responsible for this phenotype on G2 backcross
mice ([C3H x B10] x B10) to a region on mouse Chr. 4. This
locus affects virus spread in lymphocytes. We are currently
carrying out more detailed mapping and testing candidate genes
for linkage with the phenotype. The results obtained from
this combined functional/genetic approach will greatly increase
our understanding of the mechanisms which viruses use to infect
their hosts and how genetic resistance to such viruses in
the hosts occurs.
Numerous reports in recent years have implicated
a virus highly related to MMTV in human breast cancer and
patients with primary biliary cirrhosis, an autoimmune disease,
making it important to determine whether the MMTV can infect
human cells. We showed that the mouse mammary tumor virus
cell entry receptor is mouse transferrin receptor 1 (TfR1)
and that mouse and rat but not human, hamster, dog or cat
TfR1 function as MMTV entry receptors. Comparison of the 6
protein sequences revealed a small number of amino acids conserved
between mouse and rat that differ from the human, hamster,
dog and cat TfR1s. By constructing hybrid mouse/human TfR1s
we mapped the segments of the mouse receptor important for
virus infection, thus confirming that human TfR1 does not
function as an MMTV entry receptor. We also tested whether
the envelopes of the “human” MTVs had undergone
changes that altered virus tropism for human TfR1. However,
introduction of the hMTV changes into MMTV did not alter virus
tropism, making it unlikely that the mouse virus jumped species.
We are currently studying how MMTV traffics with TfR1 within
the cell during virus entry.
A final area of research in the lab is on the
role of the MMTV envelope protein in breast cancer induction.
In collaboration with John Monroe’s lab, we found that
ectopic expression of the MMTV envelope protein in normal
mammary epithelial cells resulted in phenotypic transformation
and that an immuno-tyrosine based activation motif (ITAM)
in this protein was critical to this activity. Moreover, mutation
of the ITAM motif in an infectious MMTV dramatically attenuated
its ability to cause mammary tumors, without affecting its
infectivity in vivo. ITAMs are commonly found in receptors
expressed in hematopoietic cells and are negatively regulated
by cell-type specific modulators. We speculate that uncontrolled
signaling by the envelope protein in epithelial cells, which
lack such negative modulators, is an early step in the MMTV
transformation process. Because ITAMs are found both in viral
and cellular proteins, inappropriate expression of such signaling
molecules represents a novel mechanism of transformation and
is of potential importance in developing new treatment paradigms
for breast and other cancers, especially those associated
with viruses that encode proteins that activate ITAM-mediated
signaling.
Recent
Publications
Rassa, J. and Ross, S.R. (2003). Viruses and
Toll-like receptors. Microbes and Infection, 5:961-968.
Burzyn, D., Rassa, J.C., Kim, D.C., Nepomnaschy,
I., Ross, S.R. and Piazzon, I. (2004). MMTV activates dendritic
cells through toll- like receptors. J. Virol. 78:576-584.
Katz, E., Lareef, M. H., Rassa, J.C., Russo,
J., Grande, S.M., Ross, S.R. and Monroe, J.G. (2005). An ITAM-containing
protein induces mammary epithelial cell transformation. J.
Exptl. Med., 201:431-439.
Wang, E., Albritton, L. and Ross, S.R. (2006)
Identification of the segments of the mouse transferrin receptor
required for mouse mammary tumor virus infection. J. Biol.
Chem. 281:10243-10249.
Ross, S.R., Schmidt, J.C., Katz, E., Capelli,
L., Hultine, S. Gimotty, P. and Monroe, J.G. An ITAM in the
MMTV envelope protein plays a role in virus-induced mammary
tumors. J. Virol., in press.
Lab
Rotation
Projects for 2006-2007
- Introduction of the human transferrin receptor
coding region into mouse embryonic stem cells. Mice with
targeted deletion of the transferrin receptor are embryonic
lethal. We would like to try to rescue these mice with the
human transferrin receptor. The project is to insert the
human transferrin receptor cDNA into a retroviral vector
and then infect mouse embryonic stem cells and select for
cells that contain the receptor. Techniques: subcloning,
tissue culture, DNA transfection, production of pseudoviruses,
FACS.
- Analysis of novel oncogenes in MMTV-induced
mammary tumors. We have recently carried out high through-put
analysis of MMTV integration sites in MMTV-induced tumors
and identified a number of potential novel oncogenes. The
rotation project would be to determine whether expression
of these genes is up-regulated or down-regulated in tumors
relative to normal mammary tissue. Techniques: DNA and RNA
isolation; RT-PCR; real-time PCR.
- Lab
personnel:
- Cecilia Courreges, Ph.D. – Laboratory
Manager
Chioma Okeoma, Ph.D – Postdoc
Enxiu Wang, Ph.D- Postdoc
Dionne Robinson, B.S. – Postbaccalaureate Student
Stacy Hultine, M.S. – Research Specialist
Qihua Ying, M.S. – Research Specialist
last updated 7/2006
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