Estrogenic activity of estradiol and its metabolites in the ER‐CALUX assay with human T47D breast cells

Hoogenboom, L.A.P.; Haan, Laura de; Hooijerink, Dick; Bor, Gerrit; Murk, Albertinka J.; Brouwer, Abraham

doi:10.1111/j.1600-0463.2001.tb05802.x

Cited by 15 publications

(23 citation statements)

References 17 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Our observations were consistent with the results of [15], who demonstrated that 4-OH-E2 is more oestrogenic than 2-OH-E2. In [16] it was indicated that certain oestradiol metabolites, i.e., 4-OH-E2 and 16-OH-E2, are able to mimic the effects of 17β-oestradiol on proliferation and markers of tumour metastasis.…”

Section: Action Of E2 and Its Hydroxylated Metabolites (2-oh-e2 And 4supporting

confidence: 83%

Oestrogens, Xenoestrogens and Hormone-Dependent Cancers

Ptak¹,

Gregoraszczuk²

2013

Carcinogenesis

View full text Add to dashboard Cite

Section: Action Of E2 and Its Hydroxylated Metabolites (2-oh-e2 And 4supporting

confidence: 83%

Oestrogens, Xenoestrogens and Hormone-Dependent Cancers

Ptak¹,

Gregoraszczuk²

2013

Carcinogenesis

View full text Add to dashboard Cite

“…Differences in metabolism were often responsible for the differences found between different cell lines and between cell lines and yeast-based bioassays [36,46,47]. Estrone for instance showed a REP of 0.2 in a proliferation test based on human breast cancer cells (Escreen) and the yeast estrogen bioassay, but was equally potent to E2 in a transcription activation assay based on human T47-D breast cancer cells [16,21,46]. In the ER-CALUX test with the T47-D breast cancer cells, the 17β-hydroxysteroid dehydrogenase 3 enzyme was responsible for the conversion of estrone into E2 and vice versa [46].…”

Section: Discussionmentioning

confidence: 99%

Screening of synthetic and plant-derived compounds for (anti)estrogenic and (anti)androgenic activities

Bovee¹,

Schoonen²,

Hamers³

et al. 2008

Anal Bioanal Chem

View full text Add to dashboard Cite

Recently we constructed yeast cells that either express the human estrogen receptor α or the human androgen receptor in combination with a consensus ERE or ARE repeat in the promoter region of a green fluorescent protein (yEGFP) read-out system. These bioassays were proven to be highly specific for their cognate agonistic compounds. In this study the value of these yeast bioassays was assessed for analysis of compounds with antagonistic properties. Several pure antagonists, selective estrogen receptor modulators (SERMs) and plant-derived compounds were tested. The pure antiestrogens ICI 182,780 and RU 58668 were also classified as pure ER antagonists in the yeast estrogen bioassay and the pure antiandrogen flutamide was also a pure AR antagonist in the yeast androgen bioassay. The plant-derived compounds flavone and guggulsterone displayed both antiestrogenic and antiandrogenic activities, while 3,3′-diindolylmethane (DIM) and equol combined an estrogenic mode of action with an antiandrogenic activity. Indol-3-carbinol (I3C) only showed an antiandrogenic activity. Coumestrol, genistein, naringenin and 8-prenylnaringenin were estrogenic and acted additively, while the plant sterols failed to show any effect. Although hormonally inactive, in vitro and in vivo metabolism of the aforementioned plant sterols may still lead to the formation of active metabolites in other test systems.

show abstract

“…[154][155][156][157][158] The prime motivation for studying these compounds was to search for potent STS inhibitors lacking the estrogenic effect displayed by EMATE based on the knowledge that 2-methoxyestradiol, an endogenous mammalian metabolite of estradiol, and 2-methoxyestrone are substantially less estrogenic than estrone and estradiol. 159,160 Indeed, the 2-methoxy analog 17a is a potent inhibitor of STS and shows tumor regression but no estrogenic effect in vivo. 65,154 With regard to STS inhibitory potency, 2-methoxy EMATE was approximately 7.5 times less active than EMATE as assessed in placental microsomes.…”

Section: Steroidal Arylsulfamatesmentioning

confidence: 99%

Steroid sulfatase inhibitors

Nußbaumer

Billich

2004

Medicinal Research Reviews

View full text Add to dashboard Cite

Steroid sulfatase (STS) regulates the local production of estrogens and androgens from systemic precursors in several tissues. The enzyme catalyzes the hydrolysis of the sulfate esters of 3-hydroxy steroids, which are inactive transport or precursor forms of the active 3-hydroxy steroids. STS inhibitors are expected to block the local production and, consequently, to reduce the local levels of the hormones. Therefore, they are considered as potential new therapeutic agents for the treatment of estrogen- and androgen-dependent disorders. Indications range from cancers of the breast, endometrium and prostate to androgenetic alopecia and acne. In this review, we give a comprehensive summary of the current knowledge and problems in the field of medicinal chemistry of STS inhibitors. The various types of inhibitors are presented and their structure-activity relationships are discussed. In addition to potent arylsulfamate-based, irreversible inhibitors, novel types of reversible inhibitors were recently discovered. The recent publication of the X-ray structure of STS will further boost research activities on this attractive target.

show abstract

Estrogenic activity of estradiol and its metabolites in the ER‐CALUX assay with human T47D breast cells

Cited by 15 publications

References 17 publications

Oestrogens, Xenoestrogens and Hormone-Dependent Cancers

Oestrogens, Xenoestrogens and Hormone-Dependent Cancers

Screening of synthetic and plant-derived compounds for (anti)estrogenic and (anti)androgenic activities

Steroid sulfatase inhibitors

Contact Info

Product

Resources

About