Prostate Cancer Clinical Trial
Purpose: This protocol proposes a safety and feasibility trial in patients with metastatic
prostate cancer (stages D1-D3) investigating the induction of antitumor immunity by
administration of cultured autologous peripheral blood precursor derived dendritic cells
(DC), transfected with mRNA amplified from autologous prostate tumor tissue. The feasibility
and dose-limiting toxicity of administering escalating doses of tumor RNA transfected
dendritic cells will be defined. As a secondary endpoint, the ability of tumor RNA
transfected dendritic cells to induce tumor-specific immune responses will be evaluated.
Finally, the anti-tumor effect based on PSA (biochemical) response criteria will be defined.
Background: Because prostate cancer is incurable when metastatic and conventional therapies
do not offer a clear survival benefit, new therapeutic strategies are warranted. This study
is based on the premise that clinically effective cell mediated immune responses against
prostate tumors can be elicited by activation of tumor associated antigen specific T cells.
Work performed by others and our group suggests that PSA, a protein expressed in virtually
all prostate cancers, can serve as a widely expressed candidate antigen for prostate cancer
immunotherapy. In particular, we have shown that cultured dendritic cells transfected with
mRNA encoding PSA are remarkably effective in stimulating antigen specific immunity in
vitro. Therefore, we hypothesize that administration of PSA RNA transfected DC will lead to
detectable levels of PSA specific CTL in the peripheral blood of patients with PSA
expressing metastatic prostate cancer. It is hoped that these T cell responses also have
clinical antitumor activity.
Methods: Patients will undergo percutaneous needle biopsies from either primary or
metastatic sites to obtain tumor tissue. Patients in whom sufficient tumor mRNA has been
amplified by PCR to transfect the assigned dendritic cell dose will undergo leukapheresis
and peripheral blood mononuclear cells will be cultured in vitro for 7 days with GM-CSF and
IL-4 to generate precursor derived dendritic cells. Dendritic cells will then be
cryopreserved for later use. On the day the patient returns to receive his infusion (weeks
0, 2, and 4) the dendritic cells will be thawed, reconstituted, and transfected with
amplified total tumor mRNA. Patients will receive a total of 3 treatments consisting of
combined I.V. and I.D. injections, each on study week 0, 2, and 4. Repeat leukapheresis will
be performed 2 weeks after the last dose to determine immune function. PSA levels will be
measured prior to the start of treatment and 2 weeks following the last infusion. Patients
who do not receive therapy due to a failure to produce sufficient RNA or dendritic cells
will be replaced in order to assess toxicity.
Data Analysis: 1. To determine the short and long term toxicities associated with
administration of tumor RNA dendritic cells in patients with metastatic prostate cancer. 2.
To determine feasibility of dendritic cell vaccine generation according to the proportion of
patients for whom sufficient cells are generated to provide treatment. 3. To determine the
cellular immune response to intravenous infusion of tumor RNA dendritic cells. 4. To measure
the PSA response of patients with metastatic prostate cancer to intravenous infusion of
tumor RNA dendritic cells.
;
Primary Purpose: Treatment
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