Abstract

) Human breast cancer is the predominant malignancy and the leading cause of cancer death in women from Western society. Recently, the association between human prolactin (hPRL) activity and breast cancer has been re-emphasized. In our recent studies, we have successfully developed a hPRL receptor specific antagonist by a single amino acid substitution mutation within hPRL molecule at the position 129 from Gly to Arg (hPRL-G129R). Using cell-based assays, we have demonstrated that hPRL-G129R was able to bind to hPRL receptor and block hPRL signal transduction. More importantly, we have shown that hPRL-GI29R was able to inhibit breast cancer cell proliferation through induction of apoptosis. In this study, we attempt to produce and purify hPRL-GI29R, along with hPRL (as control), and use them for in vivo studies. There are two specific aims of this proposal.
Specific aim (1) is to produce and purify greater than 70mg of hPRL and hPRL-GI29R at greater than 95 percent purity by FPLC. After hPRL and hPRL-GI29R are produced, they will be tested in vitro for their biological activities by (a) receptor binding assay; (b) STAT 5 (an intracellular signaling molecule for PRL) phosphorylation assay; and (c) apoptosis assay to ensure their quality.
Specific aim (2) is to carry out in vivo studies of hPRL-G129R using SCID mice bearing human breast cancer as model system. We choose to use two human breast cancer cells (T-47D and MCF- 7; from ATCC) and two modes of tumor inoculation for each cell lines will be used for this study (s.c to monitor the tumor development and i.p. monitor the survival rate) to ensure the in vivo experimental results. Two days after tumor cell injection, purified hPRL or hPRL-GI29R will be injected i.p. at two dose groups (1ug/g body weight and 4ug/g body weight) daily for two weeks. Following tumor development, the tumors after s.c. injection will be dissected and weighed while mice with i.p. injection of tumor cells will be followed for survival. We hope that hPRL antagonist could be used to improve the outcome of human breast cancer therapy in the near future.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Exploratory/Developmental Grants (R21)
Project #
5R21CA087093-02
Application #
6377996
Study Section
Special Emphasis Panel (ZCA1-SRRB-E (M2))
Project Start
2000-09-01
Project End
2004-08-28
Budget Start
2001-09-01
Budget End
2004-08-28
Support Year
2
Fiscal Year
2001
Total Cost
$105,000
Indirect Cost

  Institution

Name
Clemson University
Department
Microbiology/Immun/Virology
Type
Schools of Earth Sciences/Natur
DUNS #
042629816
City
Clemson
State
SC
Country
United States
Zip Code
29634

  Publications

Langenheim, John F; Chen, Wen Y (2005) Development of a prolactin receptor-targeting fusion toxin using a prolactin antagonist and a recombinant form of Pseudomonas exotoxin A. Breast Cancer Res Treat 90:281-93
Peirce, Susan K; Chen, Wen Y (2004) Human prolactin and its antagonist, hPRL-G129R, regulate bax and bcl-2 gene expression in human breast cancer cells and transgenic mice. Oncogene 23:1248-55
Beck, Michael T; Chen, Nian Y; Franek, Karl J et al. (2003) Prolactin antagonist-endostatin fusion protein as a targeted dual-functional therapeutic agent for breast cancer. Cancer Res 63:3598-604
Beck, Michael T; Peirce, Susan K; Chen, Wen Y (2002) Regulation of bcl-2 gene expression in human breast cancer cells by prolactin and its antagonist, hPRL-G129R. Oncogene 21:5047-55
Zhang, Guorong; Li, Wei; Holle, Lori et al. (2002) A novel design of targeted endocrine and cytokine therapy for breast cancer. Clin Cancer Res 8:1196-205
Chen, N Y; Holle, L; Li, W et al. (2002) In vivo studies of the anti-tumor effects of a human prolactin antagonist, hPRL-G129R. Int J Oncol 20:813-8
Ramamoorthy, P; Sticca, R; Wagner, T E et al. (2001) In vitro studies of a prolactin antagonist, hPRL-G129R in human breast cancer cells. Int J Oncol 18:25-32
Peirce, S K; Chen, W Y; Chen, W Y (2001) Quantification of prolactin receptor mRNA in multiple human tissues and cancer cell lines by real time RT-PCR. J Endocrinol 171:R1-4
Beck, M T; Holle, L; Chen, W Y (2001) Combination of PCR subtraction and cDNA microarray for differential gene expression profiling. Biotechniques 31:782-4, 786