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Evaluation of Angiogenic Potential of 1-Monocaproin Using Chick Chorioallantoic Membrane Assay

Palaniappan Maheswari1*, Kasthuri Revathi2

1Department of Biotechnology, Sathyabama University, Chennai, India

2Department of Zoology, Ethiraj College, Chennai, India

*Corresponding Author:
Maheswari P
Research Scholar, Department of Biotechnology
Sathyabama University, Jeppiaar Nagar
Rajiv Gandhi Road, Chennai 600 119
Tamil Nadu, India
Tel: 91 44 25504536/91 44 45583992
E-mail: [email protected]

Received Date: Apr 24, 2017; Accepted Date: Jun 12, 2017; Published Date: Jun 27, 2017

Citation: Maheswari P, Revathi K (2017) Evaluation of Angiogenic Potential of 1-Monocaproin Using Chick Chorioallantoic Membrane Assay. Biol Med (Aligarh) 9: 401. doi: 10.4172/0974-8369.1000401

Copyright: © 2017 Maheswari P. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

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Abstract

1-Monocaproin, a 1-monoacylglycerol, was synthesized with the reaction of glycidol by chromium-caproic fatty acid complexes and was found to be amphiphilic in nature. Synthesized 1-monocaproin was characterized by thin-layer chromatography, and the residual chromium was analyzed using inductively coupled plasma mass spectroscopy. Vascular endothelium growth factor (VEGF)-mediated angiogenesis pathways are being targeted for the development of novel drugs suitable for inhibition or stimulation of angiogenesis in various pathologies. In the chicken egg Chorioallantoic membrane (CAM) assay, 1-monocaproin exhibited VEGF-induced neovascularization in a dose-dependent manner. Synthesized 1-monocaproin was found to show the angiogenic effect at a dose concentration equivalent to VEGF at 1,000 ppm. The results thus suggest that 1-monocaproin should be considered as a useful drug candidature targeting angiogenesis in coronary artery disease, stroke, and postsurgical therapy.

Keywords

1-Monocaproin; Chorioallantoic membrane assay; Vascular endothelium growth factor; Angiogenesis

Introduction

Blood vessels constitute the fi rst organ in the embryo and form the largest network in our body but, sadly, are also oft en deadly. Upon dysregulation, the formation of new blood vessels contributes to numerous malignant, ischemic, infl ammatory, infectious, and immune disorders. Neovascularization can be understood as the growth of new capillary blood vessels in the body and is an important natural process that helps in healing and reproduction. Th e body controls neovascularization by producing a precise balance of growth and inhibitory factors in healthy tissues. When this balance is disturbed, the result is either too much or too little angiogenesis. Th e abnormal growth of blood vessels, either excessive or insuffi cient, is now recognized as a “common denominator” underlying many deadly and debilitating conditions, including cancer, skin diseases, age-related blindness, diabetic ulcers, cardiovascular disease, stroke, and many others [1]. Molecular insights into these processes are being generated at a rapidly increasing pace, off ering new therapeutic opportunities that are currently being evaluated. It represents an excellent tool for the treatment of deregulated angiogenesis-based cardiovascular diseases. It is a potent physiological process that underlies the natural manner in which our bodies respond to a diminished blood supply to vital organs, namely, the production of new collateral vessels to overcome the ischemic state [2]. A large number of preclinical studies have been performed with protein, gene, and cell-based therapies in animal models of cardiac ischemia as well as models of perpheral arterial diseases. Administration of a particular growth factor to stimulate angiogenesis in the aff ected tissues (or) organ and the protein therapy with single protein agent were not viable options to treat ischemic cardiovascular diseases [3]. Th erapeutic angiogenesis is the method of stimulation of angiogenesis where it is required but lacking. Th is technique is used to replenish the blood supply to chronic wounds to speed healing and to prevent unnecessary amputations. New research also suggests that this approach can also be used to save limbs affl icted with poor circulation and even oxygen-starved hearts [4]. Th erapeutic angiogenesis may even help to regenerate damaged (or) lost tissues in ways that were previously considered impossible such as with nerves and brain tissues. Th e modern clinical application of the principle of angiogenesis can be divided into two main areas: antiangiogenesis therapies with which angiogenesis research began and proangiogenic therapies [5]. Antiangiogenic therapies are being used to fi ght cancer and malignancies that require an abundance of oxygen and nutrients to proliferate. Proangiogenesis therapy is being explored as an option to treat cardiovascular diseases. One of the fi rst applications of proangiogenic methods in humans was a German trial using fi broblast growth factor-1 (FGF-1) for the treatment of coronary artery diseases. Clinical research in therapeutic angiogenesis is ongoing for a variety of diseases like coronary artery diseases, peripheral arterial diseases, and wound-healing disorders [6]. Th e proangiogenesis therapies can be diff erentiated into three categories, namely, (i) protein therapy, (ii) gene therapy, and (iii) cell-based therapy, which involves the implantation of specifi c cell types. Other than the above three therapies, there are a few therapies only used to induce angiogenesis. Vascular endothelium growth factor (VEGF)-mediated angiogenesis pathways are being targeted for development of novel drugs suitable for inhibition or stimulation of angiogenesis in various pathologies [7]. Th e signaling system that regulates proliferation and migration of endothelial cells during angiogenesis is mediated via key mitogen factor, namely, VEGF. Th ere remains an urgent need to develop strategies to more rapidly, inexpensively, and accurately assess the proangiogenic and antiangiogenic activities of new biologic factors and putative therapeutic agents [8]. Th e chick embryo Chorioallantoic membrane (CAM) is an extra embryonic membrane that serves as a gas exchange surface, and its function is supported by a dense capillary network [9]. Because of its extensive vascularization and easy accessibility, CAM has been used to study morphofunctional aspects of the angiogenesis process in vivo and the effi cacy and mechanism of action of pro- and antiangiogenic molecules [10]. CAM assays have been widely used to study angiogenesis [11], and the advantages of the CAM model are as follows: (i) the highly vascularized nature of the CAM greatly promotes the assessment of angiogenic property; (ii) high reproducibility; (iii) simplicity and cost effectiveness; and finally (iv) as the CAM assay is a closed system, the half-life of many new molecules tends to be much longer in comparison to animal models, allowing experimental study of potential angiogenic compounds in small quantities [12,13]. In this study, 1-monocaproin synthesized [14] through a modified process with caproic acid, glycidol, and chromium (III) chloride as a catalyst, was evaluated for a potent angiogenic compound along with VEGF (positive control) and dimethyl sulfoxide (DMSO) (negative control) through the CAM assay.

Materials and Methods

Synthesis of 1-monocaproin

Charged n-hexanoic acid kept in the 250 mL round-bottom flask in the reflux condenser was heated to 608C along with the catalyst, prepared using hexanoic acid (HA) and chromium (III) chloride hexahydrate (1:2 mol ratio), with toluene as the solvent, with continual stirring for 30 min. To this, glycidol was added slowly dropwise at 908C, and the reaction mass was maintained at 80-858C for another 120 min. The completion of the reaction was monitored by thin-layer chromatography (TLC) using the mobile phase ethyl acetate-hexane (6:4) and extracted with ethyl acetate. The organic layer was dried with sodium sulfate and concentrated under vacuum.The products of glycidol reaction, 1-monocaproin (hexanoic acid product, HAP), HA, glycidol, and a coarse material (mixture of all), were characterized by TLC using chloroform/acetone/methanol (95:4.5:0.5 v/v/v) as the mobile phase. TLC was carried out on a silica gel plate that was activated in the oven at 1508C for 30 min before use. Sample of 200 μL of each was developed on TLC plates in mobile phase, and after drying, the bands were located by viewing under 254 nm of UV light.

Angiogenesis assay using chick CAMs

CAMs of 7- to 9-day-old fertilized white Leghorn chicken eggs procured from Tamil Nadu Veterinary and Animal Sciences University, Chennai, India, were used for the assay according to a method reported previously [15]. The fertilized eggs were set upright and incubated at 378C. After 10 to 11 days of incubation, a window (10 cm2) was made in the eggshell overlying the air sac, and the CAM was exposed in each egg. Implant disks of 3 mm in diameter were made of filter paper loaded with the compounds to be tested and carefully inoculated at the junction of two blood vessels of the CAM. 1-Monocaproin was then tested at dosages of 1,000 (1 mg in 1 mL of 0.2% of DMSO), 750, 500, and 250 ppm. Then the window was sealed, eggs were incubated, and the grafts were recovered after an incubation time of 72 h. The grafts were then scored for growth and vascularization on a 0 to 4 scoring basis. A positive control VEGF, which is a potent angiogenic inducer, and a negative control DMSO were also tested simultaneously at 1,000 ppm to compare the angiogenic activity of the synthesized compound.

Results and Discussion

The synthesis of 1-monocaproin was achieved with the catalyst content of 1% by mass of charged reactants, and at 908C, yield achieved was 65% in 180 min. 1-Monocaproin synthesized with the reaction of glycidol by chromium-caprylic fatty acid complexes changes the nature of the caprylic acid from lipophilic to amphiphilic. The products of glycidol reaction, 1-monocaproin (HAP), HA, glycidol, and a coarse material (mixture of all), were characterized by TLC as shown in Figure 1, which confirmed the formation of 1-monocaproin and its yield.

biology-and-medicine-hexanoic

Figure 1: TLC picture of 1-monocaproin (HAP), hexanoic acid (HA), glycidol, and a coarse material (mixture of all)

The CAM assay has been shown to be a suitable in vivo model including many mechanisms relevant for physiological and pathological angiogenesis [16]. It was further demonstrated that different modifications of the CAM assay are versatile tools for the in vivo evaluation of small quantities (1-2 mg) of natural compounds or newly synthesized compounds, enabling the detection of possible angiogenic or antiangiogenic effects of the test compound to evaluate its property as an anticancer or angiogenic drug candidature [17,18]. Hence, the CAM assay has been found to be a most suitable tool to test 1-monocaproin at the dosages of 1,000 (1 mg in 1 mL of 0.2% of DMSO), 750, 500, and 250 ppm.

1-Monocaproin at different concentrations, along with VEGF as a positive control and DMSO as a negative control, was tested in the CAM assay for its angiogenic activity, evaluated by a score system as per Table 1, and the results of the scoring based on growth and vascularization are given in Table 2. The positive control VEGF showed the highest score, 4, wherein the granuloma was strongly vascularized and a strong starlike network of capillaries was formed around the granuloma. Among the different dose levels tested for 1-monocaproin, the dose was found to be equivalent to VEGF at a 1,000 ppm concentration. Dosedependent activity was observed with 1-monocaproin on the formation of angiogenesis. The angiogenesis effect of 1-monocaproin and the controls are shown in Figure 2.

biology-and-medicine-budding

Figure 2: HET-CAM assay: (a) shows the budding of blood vessels by VEGF at 1,000 ppm with a strong network of capillaries (positive control); (b) shows the budding of blood vessels of 1-monocaproin at 1,000 ppm with a strong network of capillaries; (c) shows the budding of blood vessels by 1-monocaproin at the concentration of 750 ppm with a weak to medium network of capillaries; (d) shows no capillary growth with DMSO (negative control)

Score Category Effects observed
4 Strong The granuloma is strongly vascularized
A starlike network of capillaries is formed around the granuloma
3 Medium The granuloma is vascularized at medium level A medium starlike network of capillaries is formed
around the granuloma
2 Weak The granuloma is weakly vascularized
A thin starlike network of capillaries is formed around the granuloma
1 Very weak The granuloma is somewhat smaller than in catego- ries 1 and 2 and only poorly vascularized
The starlike network of vessels is hardly recognizable
0 No effect No effect and no capillary growth
The network of vessels is normal (as the control)

Table 1: Score values for the evaluation of the angiogenic effect on the chorioallantoic membrane of the fertilized hen’s eggs

Test compounds Budding of blood vessels and vascularization score
1-Monocaproin (1,000 ppm) 3.67
1-Monocaproin (750 ppm) 2.33
1-Monocaproin (500 ppm) 0.67
1-Monocaproin (250 ppm) 0.33
Positive control (VEGF) 4
Negative control (DMSO) 0

Table 2: CAM assay scores of vascularization and budding of blood vessels of 1-monocaproin  and the control samples

After 72 h of incubation (see Figure 2), VEGF treatment led to a simulation with a strong network of sprouting capillaries and increased vessel density within the ring, and treatment with 1-monocaproin at the dose level of 1,000 ppm showed the formation of capillaries similar to the VEGF. No changes in vascular structure or density were observed with DMSO. One could speculate that 1-monocaproin activated the VEGF-induced biological effects on endothelial cells by stimulating the growth factor receptor interaction. VEGF is a critical endogenous proangiogenic factor that binds and activates VEGF receptor to induce angiogenesis, mitogenesis, and chemotaxis in endothelial cells. In this study also, exogenous VEGF significantly enhanced the neovascularization in the positive control groups as compared with the DMSO-treated group, evidencing its proangiogenic activity. Similarly, 1-monocaproin also exhibited neovascularization as that of VEGF. In addition, in the treatment group, a significant dose-dependent stimulation of the neovascularization was evident, evidencing its angiogenic property.

Angiogenesis, the generation of new capillaries, is a highly restricted, regulated, and self-limited activity in the healthy adult organism. The fact that pathological angiogenesis can be modulated by molecules of exogenous origin is a fast gaining credence and merits further investigation. In the present study, the CAM assay revealed that 1-monocaproin induced angiogenesis for the first time, and to conclude, the angiogenic property was best exhibited for the 1-monocaproin synthesized thorough the reaction of glycidol by the chromium-caproic fatty acid complex. The results showed that the activation of angiogenesis by 1-monocaproin is due to the stimulation of vascular endothelial cell growth, migration, and angiogenesis at a very low dose. The search and discovery of novel angiogenesis are likely to provide hope to the millions of sufferers of chronic disease and postsurgical recoveries. This work suggests that this synthesized product could be considered as a useful source of material for human health as an angiogenic agent. Because 1-monocaproin is amphiphilic in nature and Generally Regarded as Safe and (GRAS), it could be a potent drug candidature targeting coronary artery disease, stroke, chronic wound, and wound-healing formulations in combination with the existing active drug molecules. However, the underlying molecular mechanism by which 1-monocaproin stimulates the VEGF-induced neovascularization requires further studies.

Acknowledgment

We thank Bioneemtec India Private Limited, Golden Jubilee Biotech Park for Women Society, Siruseri, Chennai, India, for their facility and support.

References

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