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Synthesis and biological activity of selected cinnamic acid derivatives


Authors: Martin Gazvoda;  Slovenko Polanc
Authors place of work: Faculty of Chemistry and Chemical Technology, University of Ljubljana, Slovenia
Published in the journal: Čes. slov. Farm., 2015; 64, 294-295
Category: 44<sup>th</sup> Conference drug synthesis and analysis

Introduction

The enzymes AKR1C1 AKR1C4, members of the aldo-keto reductase superfamily, catalyse the interconversions of 3-, 17- and 20-ketosteroids with the corresponding 3α/β-, 17β-, 20α-hydroxysteroids to varying extents, using NADPH as a cofactor1). In this way they can control the ligand occupancy and trans-activation of androgen, estrogen and progesterone receptors by modulating the concentrations of the active steroids. The AKR1C enzymes are also involved in the prostaglandin and neurosteroid production and inactivation, and in the metabolism of xenobiotics. Among them, AKR1C3 preferentially acts as a 17β-ketosteroid reductase and converts a weak androgen 4-androstene-3,17-dione to a potent androgen testosterone, and estrone to a potent estrogen 17β-estradiol. AKR1C3 also catalyses the reduction of prostaglandin H2 (PGH2) into PGF2α, and PGD2 into 11β-PGF2, thereby diverting the biosynthesis of prostanoids away from the antiproliferative J-series. Catalysing these reactions, AKR1C3 represents an important target enzyme for the development of potential drugs for a treatment of the hormone dependent and hormone independent forms of cancer.

Experimental methods

General procedure for the synthesis of acids: Potassium acetate (982 mg, 10 mmol) or triethylamine (1.5 mL, 10.75 mmol) was added to a stirred mixture of the appropriate arylacetic acid (7.5 mmol), aromatic aldehyde (7.5 mmol) and acetic anhydride (3 mL, 32 mmol). The reaction mixture was stirred at 100–140 °C for 3.5‒–70 h. Then, it was cooled to rt, water was added (40 mL) and the mixture was treated with a solution of 10 M NaOH until pH 12 was reached, followed by conc. HCl (to pH 1). The resulting mixture was extracted with dichloromethane (3 . 80 mL). Organic phases were extracted with 2 M NaOH (3 . 80 mL) and water (80 mL). The combined aqueous solutions were washed with dichloromethane (100 mL) to remove the impurities and traces of starting materials, then acidified with conc. HCl (until pH was 1), and finally extracted with dichloromethane (4 . 50 mL). The organic phase was washed with brine (100 mL), dried over anhydrous sodium sulphate, evaporated to dryness and the residue was crystallized from a suitable solvent.

Cinnamic acids were assayed for their inhibition of the enzymes AKR1C1‒AKR1C3 at the Institute of Biochemistry, Faculty of Medicine, University of Ljubljana.

Results and discussion

Recently, α-methylcinnamic acid was reported as a promising inhibitor of AKR1C3 enzyme3). This prompted us to design the synthesis of a series of cinnamic acids with bulky aryl substituents on the α-position (α-arylcinnamic acids) (Fig. 1) and to evaluate their AKR1C1‒AKR1C3 inhibitory activities4).

Fig. 1. Design of α-arylcinnamic acids
Design of α-arylcinnamic acids

Acids were available with the Perkin reaction between substituted benzaldehydes and properly functionalized arylacetic acids in acetic anhydride using either potassium acetate or triethylamine as a base that led to the desired α-arylcinnamic acids (2,3-diarylpropenoic acids) as the final products (Fig. 2)4).

Fig. 2. Synthesis of α-arylcinnamic acids
Synthesis of α-arylcinnamic acids

Following the above procedure, 42 acids were synthesized, and their activities against AKR1C enzymes were evaluated, for details see4). Some of the most active and selective AKR1C3 inhibitors are presented on Figure 3.

Fig. 3. Most active and selective AKR1C3 inhibitor
Most active and selective AKR1C3 inhibitor

Conclusions

Several α-arylcinnamic acids were synthesized by the Perkin reaction between the substituted benzaldehydes and the properly functionalized arylacetic acids. They were evaluated as inhibitors of AKR1C1‒ AKR1C3. A modification of the structure revealed that the 4-methylsulfonylphenyl substituent at the position 2 of the 2,3-diarylpropenoic acid is an appropriate one to obtain a selective inhibition of AKR1C3. We found that the compound with 4-Br substituent (Fig. 2) is the best inhibitor of AKR1C3, and also shows very good selectivity. Its 4-methylphenyl and 4-ethylphenyl analogues, which exhibit a slightly lower activity against AKR1C3, are the most selective ones. Our data suggest that α-arylcinnamic acids (2,3-diarylpropenoic acids) represent a new class of selective inhibitors of AKR1C3 and may serve as a good starting point for the development of new antitumor agents for the treatment of the hormone-dependent and hormone-independent forms of prostate and breast cancers.

Conflicts of interest: none.

Dr. Martin Gazvoda

Faculty of Chemistry and Chemical Technology, University of Ljubljana

Večna pot 113, SI-1000 Ljubljana, Slovenia

e-mail: martin.gazvoda@fkkt.uni-lj.si


Zdroje

1. Penning T. M., Byrns, M. C. Steroid hormone transforming aldo-keto reductases and cancer. Ann. N. Y. Acad. Sci. 2009, 1155, 33‒42 and references therein.

2. Byrns M. C., Duan L., Lee S. H., Blair I. A., Penning T. M. Aldoeketo reductase 1C3 expression in MCF-7 cells reveals roles in steroid hormone and prostaglandin metabolism that may explain its over-expression in breast cancer. J. Steroid Biochem. Mol. Biol. 2010; 118, 177‒187.

3. Brožič P., Golob B., Gomboc N., Lanišnik-Rižner T., Gobec S. Cinnamic acids as new inhibitors of 17β-hydroxysteroid dehydrogenase type 5 (AKR1C3). Mol. Cell. Endocrinol. 2006; 248, 233‒235.

4. Gazvoda M., Beranič N, Turk S., Burja B., Kočevar M, Lanišnik-Rižner T., Gobec S., Polanc S. 2,3-Diarylpropenoic acids as selective non-steroidal inhibitors of type-5 17β-hydroxysteroid dehydrogenase (AKR1C3). Eur. J. Med. Chem. 2013, 62, 89–97.

Štítky
Pharmacy Clinical pharmacology

Článok vyšiel v časopise

Czech and Slovak Pharmacy

Číslo 6

2015 Číslo 6

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