Isolation of Adenosine and Cordysinin B from Anredera cordifolia that Stimulates CRE-Mediated Transcription in PC12 Cells

Yasushi Ohizumi; Michi Kawada; Maki Kamada; Akira Nakajima; Koji Kajima; Nobuyuki Uozumi; Yasumasa Hara; Yuanqiang Guo; Masami Ishibashi

doi:10.1055/a-1395-6510

Planta Medica International Open, Table of Contents

CC BY-NC-ND 4.0 · Planta Medica International Open 2021; 8(01): e19-e24
DOI: 10.1055/a-1395-6510

Original Papers

Isolation of Adenosine and Cordysinin B from Anredera cordifolia that Stimulates CRE-Mediated Transcription in PC12 Cells

Authors

Yasushi Ohizumi

¹Kansei Fukushi Research Institute, Tohoku Fukushi University, Aoba-ku, Sendai, Japan
Michi Kawada

¹Kansei Fukushi Research Institute, Tohoku Fukushi University, Aoba-ku, Sendai, Japan
Maki Kamada

¹Kansei Fukushi Research Institute, Tohoku Fukushi University, Aoba-ku, Sendai, Japan
Akira Nakajima

¹Kansei Fukushi Research Institute, Tohoku Fukushi University, Aoba-ku, Sendai, Japan

²Department of Applied Biology and Food Sciences, Faculty of Agriculture and Life Science, Hirosaki University, Hirosaki, Aomori, Japan
Koji Kajima

³Sankyo Co., Ltd., Fuji, Shizuoka, Japan
Nobuyuki Uozumi

⁴Department of Biomolecular Engineering, Graduate School of Engineering, Tohoku University, Sendai, Japan
Yasumasa Hara

⁵Graduate School of Pharmaceutical Sciences, Chiba University, Chuo-ku, Chiba, Japan
Yuanqiang Guo

⁶State Key Laboratory of Medicinal Chemical Biology, College of Pharmacy, and Tianjin Key Laboratory of Molecular Drug Research, Nankai University, Tianjin, China
Masami Ishibashi

⁵Graduate School of Pharmaceutical Sciences, Chiba University, Chuo-ku, Chiba, Japan

Abstract

Full Text

PDF Download

Key words

Anredera cordifolia - Basellaceae - adenosine - cordysinin B - dementia - CRE-mediated transcription

Introduction

AD is the most common neurodegenerative disorder and has become a severe social problem in advanced countries [1]. However, effective preventive and fundamental therapeutic methods for AD have not yet been established. Notably, Aβ peptide in AD patients’ brains decreases CREB signaling pathway activation to inhibit hippocampal LTP formation [2], and Aβ oligomers inhibit CREB activation in hippocampal neurons [3]. Furthermore, the CREB/CRE pathway greatly contributes to LTP, a synaptic memory model, and memory formation in vivo [[4] [5] [6] [7] [8].

Numerous natural resources have simultaneously provided useful pharmacological tools [9] and novel leading compounds for drug development [10]. We have reported that Nob, a polymethoxylated flavone from the peel of Citrus depressa, activates the CREB/CRE pathway in PC12D cells or cultured rat hippocampal neurons to exhibit memory-improving actions in various animal models of dementia [11] [12] [13] [14].

There is considerable interest in identifying safe and effective compounds from natural resources that enhance the function of CREB transcription factor coupled with CRE-mediated transcription, which could improve memory deficits in AD.

In our survey of natural resources having the increasing action of the CRE-mediated transcription activity, we found that Anredera cordifolia, like Nob, enhances this activity and reverses memory impairment caused by NMDA receptor antagonist MK-801 in mice [15]. Alternatively, A. cordifolia possesses pharmacologically interesting actions such as anti-obesity, anti-hyperlipidemia, antihypertensive, antidiabetic, antioxidant, and anti-inflammatory activities [16] [17]. Here, we unprecedentedly described that adenosine and cordysinin B are isolated as active ingredients from A. cordifolia, possessing increasing activity on CRE-mediated transcription. It is also suggested that these actions are caused by activating adenosine receptors.

Results and Discussion

AD is the most common neurodegenerative disorder showing progressive loss of memory and cognitive function. Notably, late LTP formation, a synaptic memory model, is blocked by the Aβ peptide by inhibiting the CREB signaling pathway [2]. Using a new strategy in our survey of numerous natural resources activating the CREB/CRE pathway, we found that A. cordifolia, like Nob from citrus peels, with activating actions on CRE-mediated transcription, improved MK-801-induced memory impairment [13] [14] [15] [18].

A. cordifolia leaves (202 g) were extracted using MeOH (0.4 L) for 5 days at room temperature in a stationary state to obtain the MeOH extract (47.5 g) by removing the solvent using a rotary evaporator. The MeOH extracts were fractionated by monitoring the CRE-mediated transcriptional activity using PC12 cells as illustrated in [Fig. 1]. The four layers partitioned with n-hexane, EtOAc, and BuOH had CRE-mediated transcriptional activities [12.2-fold activation (BuOH layer), 4.4-fold activation (EtOAc layer), 1.5-fold activation (n-hexane layer), and 1.3-fold activation (H₂O layer) at 30 μg/mL]. The BuOH layer (5.8 g) was subjected to silica gel 60 N column chromatography (φ45 × 420 mm, CHCl₃–MeOH system) to give fractions 1A (CHCl₃:MeOH=13:1, 0.27 L; CHCl₃:MeOH=9:1, 0.25 L), 1B (CHCl₃:MeOH=9:1, 0.15 L), 1C (CHCl₃:MeOH=9:1, 0.1 L; CHCl₃:MeOH=7:1, 0.25 L), 1D (CHCl₃:MeOH=7:1, 0.05 L; CHCl₃:MeOH=5:1, 0.3 L), 1E (CHCl₃:MeOH=5:1, 0.15 L; CHCl₃:MeOH=3:1, 0.15 L), 1F (CHCl₃:MeOH=3:1, 0.15 L), 1G (CHCl₃:MeOH=3:1, 0.10 L), 1H (CHCl₃:MeOH=3:1, 0.15 L; CHCl₃:MeOH=2:1, 0.15 L), 1I (CHCl₃:MeOH =2:1, 0.20 L; CHCl₃:MeOH=1:1, 0.15 L), 1J (CHCl₃:MeOH=1:1, 0.30 L), and 1K (CHCl₃:MeOH=1:1, 0.05 L; MeOH, 0.15 L; MeOH + 0.1% TFA, 0.15 L). Fraction 1D (CHCl₃:MeOH=7:1–5:1, 33 mg) was suspended in 5% MeOH and subjected to ODS open column chromatography (φ15 × 140 mm, MeOH–H₂O system) at once to give subfractions 2A (H₂O, 0.02 L), 2B (5% MeOH, 0.02 L), 2C (10% MeOH, 0.02 L), 2D (15% MeOH, 0.02 L), 2E (20% MeOH, 0.02 L), 2F (25% MeOH, 0.02 L), 2G (40% MeOH, 0.02 L), 2H (50% MeOH, 0.02 L), 2I (MeOH, 0.02 L), and 2J (MeOH + 0.1% HCOOH, 0.02 L). Subfraction 2E (20% MeOH, 0.7 mg) was regarded as compound 2 ([Fig. 2]). A part of fraction 1H (CHCl₃: MeOH=3:1–2:1, 671 mg of 681 mg) was subjected to silica gel PSQ 100B column chromatography (φ25 × 160 mm, CHCl₃–MeOH system) to give subfractions 3A-3I. A part of subfraction 3E (CHCl₃: MeOH=5:1, 54 mg of 64 mg) was subjected to HPLC [COSMOSIL Cholester (φ10.0 × 250 mm); eluent: 20% MeOH; flow rate: 5.0 mL/min; UV detection: 254 nm] to give compound 1 (4.4 mg, t _R 4.7 min) ([Fig. 2]).

Fig. 1 Scheme for isolation of pharmacologically active compounds from A. cordifolia.

Fig. 2 Chemical structures of compounds 1 (adenosine) and 2 (cordysinin B) from the MEAC.

DMSO and Nob served as the negative and positive controls, respectively, in measuring CRE-mediated transcriptional activity. As can be seen in [Fig. 3], MEAC induces a powerful increasing action on CRE-mediated transcription in PC12 cells. Also, the BuOH layer showed the strongest activity among the four layers and then was chromatographed on silica gel to afford the active compounds 1 and 2. The physicochemical properties of the active compounds 1 and 2 properly correspond to those of adenosine and cordysinin B, respectively (Table S1 and S2) [19] [20]. Cordysinin B was previously isolated from Cordyceps sinensis [20]. Therefore, it is concluded that the major active ingredients of A. cordifolia are adenosine and cordysinin B, respectively.

Fig. 3 Increasing activities of the MEAC and the layer of n-hexane (Hex), ethyl acetate (EtOAc), n-buthanol (BuOH), or water (H₂O) on CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). For some data points, error bars are smaller than the symbol size.

[Fig. 4] indicates that introducing a methyl group into the OH group at the C-2′ position of adenosine decreases the CRE-mediated transcription activity approximately 100 times. Therefore, these results suggest that the OH group is important for developing the activity.

Fig. 4 Concentration-dependent effects of adenosine a, cordysinin B b, and nobiletin c on CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). For some data points, error bars are smaller than the symbol size.

To demonstrate the mechanisms responsible for CRE-mediated transcription induction by adenosine and cordysinin B, we used adenosine A receptor antagonists CGS 15943 (a nonselective adenosine A receptor antagonist), DPCPX (an adenosine A₁ receptor antagonist), SCH 58261 (an adenosine A_2A receptor antagonist), MRS 1754 (an adenosine A_2B receptor antagonist), and MRS 1523 (an adenosine A₃ receptor antagonist). CRE-mediated transcription induced by adenosine and cordysinin B was blocked by pretreating with CGS 15943, DPCPX, SCH 58261, or MRS 1754, although the effect of MRS 1754 on adenosine-induced CRE-mediated transcription was weak ([Fig. 5]). In contrast, MRS 1523 did not affect CRE-mediated transcription induced by adenosine or cordysinin B. These results suggest that adenosine and cordysinin B induce CRE-mediated transcription, at least in part, by A₁, A_2A, and A_2B receptors.

Fig. 5 Effects of adenosine receptor antagonists on adenosine- and cordysinin B-induced enhancement of CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). ^***P<0.001 vs. DMSO-treated control; ^###p<0.001 vs. adenosine alone-treated group; ⁺⁺⁺p<0.001 vs. cordysinin B alone-treated group.

Conclusively, adenosine and cordysinin B are isolated active ingredients from A. cordifolia and possess the activity to induce CRE-mediated transcription, an important event for memory formation. It is also suggested that these actions are induced, at least in part, by adenosine A₁, A_2A, and A_2B receptors, but not A₃ receptor.

Materials and Methods

Plant material

A. cordifolia leaves were collected from the hothouse of Sankyo Co., Ltd. in Fuji, Japan from May 2015 to July 2016. The plant material was identified by Dr. Koji Kajima. A voucher specimen was deposited at Sankyo Co., Ltd. (SS-U001). A. cordifolia, a perennial Basellaceae native to South America, has been used as a traditional medicine in China and Japan.

General experimental procedures in chemistry

An ECZ-600 spectrometer (JEOL) was used for NMR spectroscopy and the chemical shift of the NMR solvent was used as an internal standard. An HPLC system (Shimadzu) comprising an SCL-10AVP system controller, LC-20AD pump, DGU-12A online degasser, SIL-20A, CTO-10ASVP column oven, SIL-20A autosampler, SPD-M20A PDA detector, and CLASS-VP software was used. The following adsorbents were used for purification: silica gel 60 F254 (0.25 mm; Merck) and silica gel 60 RP-8 F254 S (0.25 mm; Merck) for analytical TLC; Silica gel 60 N (Kanto), silica gel PSQ 100B, and Chromatrex ODS (Fuji Silysia chemical) for column chromatography; COSMOSIL Cholester (φ10.0 × 250 mm; Nacalai Tesque) for HPLC.

Reagents

CGS 15943 was obtained from Cayman Chemical. DPCPX, SCH 5826, MRS 1754, and MRS 1523 were purchased from Abcam. Adenosine (purity ≥ 99%) and cordysinin B (2’-O-Methyl Adenosine) (purity ≥ 98%) were from Sigma-Aldrich and Toronto Research Chemicals, respectively. Nob was extracted and isolated from C. depressa peels as described previously [11] [12]. The purity of Nob was confirmed to be almost 100%.

Culture of rat pheochromocytoma (PC12) cells

PC12 cells were grown in DMEM supplemented with 10% heat-inactivated horse serum (Gibco by Life Technologies), 5% heat-inactivated fetal bovine serum (Gibco), and 1% penicillin/streptomycin (Gibco) at 37°C in a humidified atmosphere of 95% air and 5% CO₂.

Measurements of cyclic AMP-response element-mediated transcriptional activity in PC12 cells

Transient transfection and the reporter gene assay were prepared as described previously [11]. PC12 cells cultured in 96-well plates (4 × 10⁴/well) were transfected for 5 h with 0.2 mg of the reporter plasmid pCRE (Clontech) and 0.04 mg of the transfection efficiency Renilla luciferase phRG-TK plasmid (Promega) using LipofectAMINE (Invitrogen) according to the manufacturer’s instructions. After transfection, the medium was replaced with a fresh medium containing advanced DMEM, 1% horse serum (Gibco), and 1% fetal bovine serum (Gibco), and the cells were incubated overnight. After incubation, the cells were stimulated for 5 h with MEAC, adenosine, or cordysinin B. In the reporter gene assay, commercially available adenosine standard (Sigma-Aldrich, catalog A4036) and cordysinin B standard (Toronto Research Chemicals, catalog M276150) were used. For experiments using adenosine receptor antagonists, the cells were preincubated with CGS 15943(3 μM), DPCPX (0.5 μM), SCH 58261 (3 nM), MRS 1754 (30 μM), or MRS 1523 (1 μM) for 30 min before stimulation and then stimulated for 5 h with adenosine or cordysinin B in the presence of an individual antagonist. Luminescence was measured using a Dual-Luciferase Reporter Assay System according to the manufacturer’s instructions (Promega). All treatments were performed in quadruplicate on at least three independent cultures.

Statistical analysis

The results are expressed as the mean±SEM. Data were analyzed using one-way analysis of variance (ANOVA), followed by Tukey-Kramer test, and p<0.05 was considered statistically significant difference.

Supporting information

1H NMR and MS spectra of compound 1, 1H and 13C NMR and MS spectra of compound 2, and tables for comparison of the physicochemical properties between compound 1 and adenosine and those between compound 2 and cordysinin B are available as Supporting information.

References

References
1 Huang Y, Mucke L. Alzheimer mechanisms and therapeutic strategies. Cell 2012; 148: 1204-1222
2 Vitolo OV, Sant'Angelo A, Costanzo V, Battaglia F, Arancio O, Shelanski M. Amyloid beta-peptide inhibition of the PKA/CREB pathway and long-term potentiation: reversibility by drugs that enhance cAMP signaling. Proc Natl Acad Sci USA 2002; 99: 13217-13221
3 Ma QL, Harris-White ME, Ubeda OJ, Simmons M, Beech W, Lim GP, Teter B, Frautschy SA, Cole GM. Evidence of Abeta- and transgene-dependent defects in ERK-CREB signaling in Alzheimer's models. J Neurochem 2007; 103: 1594-1607
4 Frey U, Huang YY, Kandel ER. Effects of cAMP stimulate a late stage LTP in hippocampal CA1 neurons. Science 1993; 260: 1661-1664
5 Impey S, Mark M, Villacres EC, Poser S, Chavkin C, Storm DR. Induction of CRE-mediated gene expression by stimuli that generate long-lasting LTP in area CA1 of the hippocampus. Neuron 1996; 16: 973-982
6 Abel T, Nguyen PV, Barad M, Deuel TA, Kandel ER, Bourtchouladze R. Genetic demonstration of a role for PKA in the late phase of LTP and in hippocampus-based long-term memory. Cell 1997; 88: 615-626
7 Sweatt JD. Mitogen-activated protein kinases in synaptic plasticity and memory. Curr Opin Neurobiol 2004; 14: 311-317
8 Kandel ER. The molecular biology of memory: cAMP, PKA, CRE, CREB-1, CREB-2, and CPEB. Mol Brain 2012; 5: 14
9 Ohizumi Y. Application of physiologically active substances isolated from natural resources to pharmacological studies. Jpn J Pharmacol 1997; 73: 263-289
10 Li JW, Vederas JC. Drug discovery and natural products: End of an era or an endless frontier?. Science 2009; 325: 161-165
11 Nagase H, Omae N, Omori A, Nakagawasai O, Tadano T, Yokosuka A, Sashida Y, Mimaki Y, Yamakuni T, Ohizumi Y. Nobiletin and its related flavonoids with CRE-mediated transcription-stimulating and neuritegenic activities. Biochem Biophys Res Commun 2005; 337: 1330-1336
12 Nagase H, Yamakuni T, Matsuzaki K, Maruyama Y, Kasahara J, Hinohara Y, Kondo S, Mimaki Y, Sashida Y, Tank AW, Fukunaga K, Ohizumi Y. Mechanism of neurotrophic action of nobiletin in PC12D cells. Biochemistry 2005; 44: 13683-13691
13 Nakajima A, Ohizumi Y, Yamada K. Anti-dementia activity of nobiletin, a citrus flavonoid: A review of animal studies. Clin Psychopharmacol Neurosci 2014; 12: 75-82
14 Nakajima A, Ohizumi Y. Potential benefits of nobiletin, a citrus flavonoid, against Alzheimer’s disease and Parkinson’s disease. Int J Mol Sci 2019; 20: 3380
15 Nakajima A, Hachiro M, Kajima K, Ohizum Y. Anredera cordifolia extract improves MK-801-induced memory impairment in mice. Pharmacometrics 2020; 98: 27-30
16 Yuniarti WM, Lukiswant BS. Effects of herbal ointment containing the leaf extracts of Madeira vine (Anredera cordifolia (Ten.) Steenis) for burn wound healing process on albino rats. Vet World 2017; 10: 808-813
17 Leliqia NPE, Sukandar EY, Fidrianny I. Overview of efficacy, safety and phytochemical study of Anredera cordifolia (TEN.) steenis. Pharmacologyonline 2017; 1: 124-131
18 Ohizumi Y. [A new strategy for prevention and finctional therapeutic methods for dementia --approach using natural products]. . Yakugaku Zasshi 2015; 135: 449-464
19 Ciuffreda P, Casati S, Manzocchi A. Complete 1H and 13C NMR spectral assignment of a α- and β-adenosine, 2'-deoxyadenosine and their acetate derivatives. Magn Reson Chem 2007; 45: 781-784
20 Yang ML, Kuo PC, Hwang TL, Wu TS. Anti-inflammatory principles from Cordyceps sinensis. J Nat Prod 2011; 74: 1996-2000

Figures

Fig. 1 Scheme for isolation of pharmacologically active compounds from A. cordifolia.

Fig. 2 Chemical structures of compounds 1 (adenosine) and 2 (cordysinin B) from the MEAC.

Fig. 3 Increasing activities of the MEAC and the layer of n-hexane (Hex), ethyl acetate (EtOAc), n-buthanol (BuOH), or water (H₂O) on CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). For some data points, error bars are smaller than the symbol size.

Fig. 4 Concentration-dependent effects of adenosine a, cordysinin B b, and nobiletin c on CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). For some data points, error bars are smaller than the symbol size.

Fig. 5 Effects of adenosine receptor antagonists on adenosine- and cordysinin B-induced enhancement of CRE-mediated transcription in PC12 cells. Data are shown as the mean±SEM (n=4). ^***P<0.001 vs. DMSO-treated control; ^###p<0.001 vs. adenosine alone-treated group; ⁺⁺⁺p<0.001 vs. cordysinin B alone-treated group.

Supplementary Material

Supplementary Material (PDF)