Neuroblastoma Clinical Trial
Official title:
The Role of Aromatic Hydrocarbon Receptor in the Tumorigenesis of Neuroblastoma and Its Relationship With MYCN Expression
Neuroblastoma (NB) is the most common malignant tumor of infancy. Approximately 60% of NB
patients are clinically diagnosed as the stage IV disease and have a very poor prognosis
with the 5-year survival rate no more than 30%. Molecular markers of NB have great impacts
on the tumor behavior. MYCN amplification is the most well-known marker to predict a poor
outcome in NB patients. However, how MYCN affects the NB cell behavior remains unknown. In
our preliminary studies, we performed a genome-wide analysis of the differential gene
expression in 10 NB tumors with MYCN amplification and 10 with normal MYCN copy number. We
found that aromatic hydrocarbon receptor (AHR) reversely correlated with the MYCN
expression. This relationship was verified in 83 NB tumor samples. In addition, positive AHR
expression by immunostaining of NB tumors predicted a favorable prognosis. These lines of
evidence demonstrate that AHR not only relates to the MYCN expression but also plays an
important role in the tumorigenesis of NB. Therefore in this project we aim at further
studying the relationship between AHR and MYCN. In addition, the possible role of AHR in the
tumorigenesis of NB will be clarified. Specifically, we propose a 3-year project with the
following three aims:
Aim I. Determine the molecular relationship between AHR and MYCN expression. AHR has been
shown to suppress the E2F1 expression. E2F1 reversely has been found to upregulate the
expression of MYCN. In our preliminary microarray study, we also found that the expression
E2F1 positively correlated with the MYCN expression but inversely correlated with the
expression of AHR. Therefore, NB cells will be transfected with AHR expression vector or AHR
siRNA, then the associated E2F1 and MYCN expression will be examined to clarify if AHR could
regulate MYCN expression via E2F1. Furthermore, the E2F1 levels will also be manipulated to
determine if the effect of AHR on MYCN depends on E2F1. In addition, the E2F1 expression in
NB tumor samples will also be examined to clarify its in vivo role.
Aim II. Determine the effect of AHR expression on the NB cell behavior. The baseline AHR
expression levels in several NB cell lines will be examined. AHR is then overexpressed by
gene transfection in NB cells. The cell proliferation, migration, and differentiation after
AHR overexpression are evaluated. Furthermore the AHR expression in normal neuron cells is
also examined, and suppressed by siRNA to if downregulation of AHR could lead to cancer
development.
Aim III. Determine if AHR could be a target of gene therapy for NB. NB cells with either
normal MYCN or MYCN amplification before and after AHR gene transfection are inoculated into
nude mice to demonstrate the effect of AHR expression on NB cells behavior in vivo. AHR is
then transfected into the wild type NB tumor to see if the tumor growth could be suppressed
by AHR expression. Then wild type tumor and tumors transfected with AHR are subjected
microarray analysis to compare with the human tumor data set for evaluation of gene
expression changes along with differential AHR expression. Altogether, our studies will not
only establish the relationship between AHR and MYCN, but also allow us to depict the
functional role of AHR-MYCN interaction in the tumorigenesis of NB.
n/a
Observational Model: Cohort, Time Perspective: Retrospective
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