Differential growth factor responses of epithelial cell cultures derived from normal human prostate, benign prostatic hyperplasia, and primary prostate carcinoma

Chopra, Dharam P.; Grignon, David J.; Joiakim, Aby; Mathieu, Patricia; Mohamed, Anwar N.; Sakr, Wael; Powell, Isaac J.; Sarkar, Fazlul H.

doi:10.1002/(sici)1097-4652(199611)169:2<269::aid-jcp6>3.0.co;2-m

Cited by 32 publications

(20 citation statements)

References 25 publications

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“…This raises the issue of when using surgical material whether what grows out in lowCa 2+ -SFD medium are truly cancer cells as opposed to highly proliferative transit-amplifying cells derived from basal epithelium of normal glands contaminating the starting cancerous tissue. This latter possibility is supported by the demonstration that (a) such low-Ca 2+ -SFD medium cultures usually are not capable of being propagated beyond 10 passages although they are derived from cancerous tissue (25), (b) they usually lack molecular and karyotypic changes (e.g., 8p…”

Section: +mentioning

confidence: 98%

“…Based on this success, many groups are using variations of lowCa 2+ -SFD medium containing known growth factors [e.g., PrEBM complete medium or keratinocyte serum-free medium (K-SFM) complete medium from Invitrogen (Carlsbad, CA) in an attempt to grow sufficient numbers of prostate cancer cells from surgical material obtained at radical prostatectomy for molecular analysis and to establish new serially passageable prostate cancer cell lines (20)(21)(22)(23)(24)(25)(26)(27)(28)(29)(30). Such a serum-free approach is favored because FCS contains a variety of undefined, and thus hard to standardize, factors in addition to its potent ability to stimulate growth to unwanted prostate stromal cells (i.e., fibroblasts and smooth muscle cells).…”

Section: +mentioning

confidence: 99%

“…Such a serum-free approach is favored because FCS contains a variety of undefined, and thus hard to standardize, factors in addition to its potent ability to stimulate growth to unwanted prostate stromal cells (i.e., fibroblasts and smooth muscle cells). Using such a low-Ca 2+ -SFD medium approach, it has been claimed that pure populations of prostate cancer cells can be grown and propagated from starting prostate cancer tissue (25)(26)(27)(28). In contrast to these low-Ca 2+ -SFD medium approaches, all of the presently available, serially propagated human prostate cancer cell lines (i.e., DU-145, PC-3, LNCaP, C4-2B, LAPC-4, CWR22-Rv1, CWR-R1, MDA-PCA-2A, MDA-PCA-2B, DuCap, and VCap) were originally established with and are maintained in 10% FCS containing medium whose Ca 2+ is between 650 and 1,860 Amol/L (18).…”

Section: +mentioning

confidence: 99%

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Role of Notch-1 and E-Cadherin in the Differential Response to Calcium in Culturing Normal versus Malignant Prostate Cells

Dalrymple

Antony

et al. 2005

Cancer Research

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A panel of expression markers was validated and used to document that, when radical prostatectomy specimens are cultured in low (i.e., <260 Mmol/L)-calcium (Ca 2+ )-serum-free, growth factor-defined (SFD) medium, what grows out are not prostatic cancer cells but basally derived normal transitamplifying prostatic epithelial cells. The selective outgrowth of the normal transit-amplifying versus prostatic cancer cells is due to the differential effect of low-Ca 2+ medium on the structure of Notch-1 and E-cadherin signaling molecules. In low-Ca 2+ medium, Notch-1 receptor is conformationally in a constitutively active, cell autonomous form not requiring reciprocal cell-cell (i.e., ligand) interaction for signaling. Such signaling is required for survival of transit-amplifying cells as shown by the death of transit-amplifying cells induced by treatment with a series of chemically distinct ;-secretase inhibitors to prevent Notch-1 signaling. Conversely, in lowCa 2+ medium, E-cadherin is conformationally inactive preventing cell-cell homotypic interaction, but low cell density nonaggregated transit-amplifying cells still survived because Notch-1 is able to signal cell autonomously. In contrast, when medium Ca 2+ is raised to >400 Mmol/L, Notch-1 conformationally is no longer constitutively active but requires cell-cell contact for reciprocal binding of Jagged-1 ligands and Notch-1 receptors between adjacent transit-amplifying cells to activate their survival signaling. Such cell-cell contact is enhanced by the elevated Ca 2+ inducing an E-cadherin conformation allowing homotypic interaction between transit-amplifying cells. Such Ca 2+ -dependent, E-cadherin-mediated interaction, however, results in cell aggregation, stratification, and inhibition of proliferation of transit-amplifying cells via contact inhibition-induced up-regulation of p27/kip1 protein.In addition, transit-amplifying cells not contacting other cells undergo squamous differentiation into cornified (i.e., 1% SDS insoluble) envelopes and death in the elevated Ca 2+ medium. Stratification and contact inhibition induced by elevated Ca 2+ are dependent on E-cadherin-mediated homotypic interaction between transit-amplifying cells as shown by their prevention in the presence of a cell-impermanent, E-cadherin neutralizing antibody. In contrast to growth inhibition of normal transit-amplifying cells, supplementation of low-Ca 2+ -SFD medium with 10% FCS and raising the Ca 2+ to >600 Mmol/L stimulates the growth of all prostate cancer cell lines tested.Additional results document that, at physiologic levels of Ca 2+ (i.e., >600 Mmol/L), prostatic cancer cells are not contact inhibited by E-cadherin interactions and Notch-1 signaling is no longer required for survival but instead becomes one of multiple signaling pathways for proliferation of prostatic cancer cells. These characteristic changes are consistent with prostate cancer cells' ability to metastasize to bone, a site of high-Ca 2+ levels. (Cancer Res 2005; 65(20): 9269-79)

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Section: +mentioning

confidence: 98%

Section: +mentioning

confidence: 99%

Section: +mentioning

confidence: 99%

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Role of Notch-1 and E-Cadherin in the Differential Response to Calcium in Culturing Normal versus Malignant Prostate Cells

Dalrymple

Antony

et al. 2005

Cancer Research

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“…NHP1-NHP6 cells were cultured in serum-and androgen-free, PrEBM medium (Clonetics) supplemented with insulin, EGF, hydrocortisone, bovine pituitary extract, and cholera toxin, and used at passages 3-7 (Chopra et al, 1996;Tang et al, 1998Tang et al, , 2002Bhatia et al, 2003). PCa cell lines, PPC-1, PC3, LNCaP, and Du145, were cultured in RPMI 1640 supplemented with 10% heat-inactivated fetal bovine serum (FBS) and antibiotics.…”

Section: Cells and Reagentsmentioning

confidence: 99%

Evidence that Sp1 positively and Sp3 negatively regulate and androgen does not directly regulate functional tumor suppressor 15-lipoxygenase 2 (15-LOX2) gene expression in normal human prostate epithelial cells

et al. 2004

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In this project, we studied the gene regulation of 15-lipoxygenase 2 (15-LOX2), the most abundant arachidonate-metabolizing LOX in adult human prostate and a negative cell-cycle regulator in normal human prostate (NHP) epithelial cells. Through detailed in silico promoter examination and promoter deletion and activity analysis, we found that several Sp1 sites (i.e., three GC boxes and one CACCC box) in the proximal promoter region play a critical role in regulating 15-LOX2 expression in NHP cells. Several pieces of evidence further suggest that the Sp1 and Sp3 proteins play a physiologically important role in positively and negatively regulating the 15-LOX2 gene expression, respectively. First, mutations in the GC boxes affected the 15-LOX2 promoter activity. Second, both Sp1 and Sp3 proteins were detected in the protein complexes that bound the GC boxes revealed by electrophoretic mobility shift assay. Third, importantly, inhibition of Sp1 activity or overexpression of Sp3 both inhibited the endogenous 15-LOX2 mRNA expression. Since 15-LOX2 is normally expressed in the prostate luminal epithelial cells, we subsequently explored whether androgen/androgen receptor may directly regulate its gene expression. The results indicate that androgen does not directly regulate 15-LOX2 gene expression. Together, these observations provide insight on how 15-LOX2 gene expression may be regulated in NHP cells.

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“…NHPl, NHP3, NHP4, and NHP6 cells were obtained from Clonetics (Walkersville, MD), and NHP2 and NHP5 cells were generated as previously described (7)(8)(9). These cells were cultured in serum-free, PrEBM medium (Clonetics) …”

Section: Methodsmentioning

confidence: 99%

Arachidonate 15-Lipoxygenase 2 as an Endogenous Inhibitor of Prostate Cancer Development

Tang¹

2006

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Differential growth factor responses of epithelial cell cultures derived from normal human prostate, benign prostatic hyperplasia, and primary prostate carcinoma

Cited by 32 publications

References 25 publications

Role of Notch-1 and E-Cadherin in the Differential Response to Calcium in Culturing Normal versus Malignant Prostate Cells

Role of Notch-1 and E-Cadherin in the Differential Response to Calcium in Culturing Normal versus Malignant Prostate Cells

Evidence that Sp1 positively and Sp3 negatively regulate and androgen does not directly regulate functional tumor suppressor 15-lipoxygenase 2 (15-LOX2) gene expression in normal human prostate epithelial cells

Arachidonate 15-Lipoxygenase 2 as an Endogenous Inhibitor of Prostate Cancer Development

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