Saturday, January 25, 2020

Standardization of Anti-diabetic Poly Herbal Formulation

Standardization of Anti-diabetic Poly Herbal Formulation 1. Introduction Now-a-days most of developed as well as developing countries use Ayurvedic medicines then they uses it in past. They avoid use of allopathic drugs because of high risk of adverse effects. So, for the sake of community it is important to standardize the dosage form available in market. Standardization of formulation is evidence that the formulation contains constituents which it says to be contained. In present work formulation containing Gymnemic acid and Resveratrol has been studied. This formulation is anti-diabetic. Gymnemic Acid (GYM) is major constituent isolated from leaves of plant Gymnema Sylvester belonging to family Asclepiadacea. (1) Plant has a property of masking the sugar test so it is known as â€Å"GURMAR†. Gymnemic acid is a triterpenoid saponin found in the leaves of Gymnema Sylvester. (2) Many studies have shown that oral administration of Gymnema extract reduces serum glucose level and improves glucose tolerance in mildly diabetic rats. (3) Administration of water extract of Gymnema sylvestre leaves was found to increase serum insulin level suggesting its insulin releasing effect. (4) Number of beta cells within pancreatic tissue were increased which suggests a restorative effect of the Gymnema extract on pancreatic tissue. (5) So, from above it is now known that Gymnemic acid has the ability to decrease blood glucose level in diabetic patient which ultimately relives Diabetes. Resveratrol (RES) (3,4†²,5-trihydroxy-trans-stilbene) is polyphenolic constituent isolated from plant Polygonum Cuspidatum belonging to family Polygnaceae. (6) It has been reported that Resveratrol has a variety of biological and pharmacological effects including antioxidant, anti-inflammatory, antiplatelet, anticarcinogenic effects, modulation of lipid metabolism and cardioprotection. (7) In pancreatic ÃŽ ²-cells, insulin secretion is linked to the oscillations in membrane potential, intracellular Ca2+ and metabolism. The variations in the ATP/ADP ratio control the conductance of ATP-dependent K+ channels leading to depolarization and periodic influx of Ca2+. The resultant membrane depolarization activates voltage dependent L-type Ca2+ channels and triggers intracellular Ca2+ release, elevating intracellular Ca2+ both in the cytosolic compartment and within the mitochondria, and thereby initiating insulin secretion. (8) From the survey of various literatures it is found that Gymnemic acid has been estimated by various analytical techniques like HPTLC, HPLC Gravimetery. (9) While Resveratrol had been estimated by HPLC and spectrometric techniques. (10) Not a single method is reported for the estimation of both constituents simultaneously. Present work has been focused on estimation of both constituents simultaneously. Here estimation of both constituents was done by UV-Visible spectrometry and HPTLC. For estimation of both constituents simultaneously UV-visible Spectrophotometric and HPTLC methods were developed and validated. Figure 1: Gymnemic acid Table 1: Gymnemic acid Group Figure 2: Resveratrol 2. Experimental Chemical Reagents Gymnemic acid relative Standard was extracted from the formulation. This relative standard was compared with standard obtained from Clearsynth TM Private Ltd (Andheri (w), Mumbai, India) . Then the prepared relative standard was used for methods. Same way, Resveratrol was extracted from formulation and then compared with standard Sigma-Aldrich constituent. Marketed formulation here used was Resveratrol plus (with Gymnemic acid) {Zenith Nutrition’s} containing 100mg Resveratrol and 500 mg Gymnemic acid per 2 capsules. All reagents for UV-Visible Spectrophotometry and HPTLC are Methanol, Chloroform, Ethanol, Glacial Acetic Acid, water and Benzoyl Chloride. Methanol, Chloroform and Ethanol used were analytical grade purchased from merk solutions. Triple distill water was made in laboratory by distillation assembly. Benzoyl Chloride was purchased from SD fines Chemicals. Instruments UV-Visible Spectrophotometric was developed on a Shimadzu UV-Vis double beam spectrophotometer, model 2400 PC series, with spectral width of 1 nm, wavelength accuracy of 0.5nm and a pair of 10 mm matched quartz cells (Shimadzu , Japan). The HPTLC instrumentation consisted of a Linomat V sample applicator with 100  µL Hamilton syringe and a TLC III scanner controlled by WinCATS software (Camag, Muttenz, Switzerland) Merck TLC plates coated with 60F254 silica gel on aluminum sheets were used as stationary phase. The plates were developed in a Camag 10 x 10 cm twin through chamber that was previously saturated for 20 minutes with mobile phase. Spectrometric Conditions GYM didn’t contain chromophore in structure so it has to be derivatized for UV-Visible detection. Benzoyl Chloride was used as derivatizing agent. The solutions of GYM RES were scanned in the spectrum mode from 200 to 400 nm, and from that 303nm for Gymnemic acid determination, 318.4 nm for Resveratrol determination and 349 nm for isoabsorptive point for Q ratio method were selected for simultaneous estimation. Chromatography Condition The solutions were spotted in the form of hands of 5 mm width on pre-coated silica gel 60F254 aluminum plates using a Camag 100  µL sample applicator syringe. They were activated at 110 oC in an oven for 20 minutes before sample application. A constant application rate 0.1 µL/s was applied and bandwidth was 9 mm between two bands. Spotted plates were developed in twin through chamber which is previously saturated for 20 minutes with mobile phase containing Chloroform: Methanol: Glacial acetic acid (13: 4: 0.5 %). The plates were developed for 8 cm run length. The plates were dried by hair dryer and then post derivatization done by dipping plates in Vanillin-Sulphuric acid solution. Then it is heated in hot air oven at 105oC for 5 minutes. Then plates were scanned at 575nm in TLC III scanner. Preparation of solutions Preparation of Standard solution for UV Resveratrol relative standard 10 mg was accurately weighed which is transferred to 10 ml clean volumetric flask. This much quantity was dissolved in 10 ml of ethanol to produce 1000 µg/ ml standard stock solution. From standard stock solution 1 ml is transferred to another 10 ml of volumetric flask and volume was made up with methanol to produce 100  µg/ ml working standard stock solution. Gymnemic acid relative standard 100 mg was accurately weighed which is transferred to 10 ml clean volumetric flask. This much quantity was dissolved in 10 ml of triple distill water to produce 10000  µg/ ml standard stock solution. From standard stock solution 1 ml was transferred to 10 ml volumetric flask diluted with methanol to produce 1000  µg/ ml working standard solution. Benzoyl chloride was diluted in ethanol first and then in methanol lastly to produce 125  µg/ ml solution which was used as derivatizing solution. Preparation of sample solution for UV 10 capsule’s shells were removed and powders from those capsules were mixed and from that weight equivalent to 10 mg Resveratrol and 50 mg Gymnemic acid was weighed accurately and transferred to 10 ml of volumetric flask volume made up with mixture of ethanol: water (1:1). From this solution 1 ml solution was taken diluted with mixture of ethanol: water (1:1).this solution is working sample solution further dilution done by the same mixture. Preparation of standard solution for HPTLC Resveratrol relative standard 20 mg and Gymnemic acid relative standard 100 mg was accurately weighed and transferred to two different 10 ml volumetric flask respectively in which weighed quantity was dissolved in 10 ml ethanol : water (1:1) mixture to produce RES 2000  µg/ ml and GYM 10000  µg/ ml standard stock solution. From these solution 5 ml solution was transferred to 10 ml volumetric flask diluted with ethanol: water (1:1) up to 10 ml to produce RES 1000  µg/ ml and GYM 5000  µg/ ml working standard stock solution. Preparation of sample solution for HPTLC 10 capsule’s shells were removed and powders from those capsules were mixed from that weight equivalent to 20 mg RES and 100 mg Gym was weighed. That much amount of powder was accurately transferred to 10 ml volumetric flask and dissolved in ethanol: water (1:1) mixture. From this solution 5 ml was taken and filtered with 0.45  µm filter sized syringe filter. This solution was then diluted with mixture of ethanol: water (1:1) up to 10 ml solution to produce RES 1000  µg/ ml equivalent and GYM 5000  µg/ ml equivalent. Assay method validation Preparation of calibration curve For UV-visible Spectrophotometric method individual solutions were prepared in methanol from working standard stock solution to produce 5-25  µg/ ml RES and 25- 125  µg/ ml GYM solution. Benzoyl chloride 10  µL was added to each solution. Then these solutions were analyzed in methanol at three different wavelengths at 303 nm, 318.4 nm and 349 nm. Calibration curve here made up was absorbance v/s concentration. For HPTLC method different aliquots of were taken from standard stock solution to make final concentration of RES 1000  µg/ ml and GYM 5000  µg/ ml in the same solution. Then different aliquots were spotted on activated TLC plate. The concentration of RES was varied between (5-25)  µg/ spot while for GYM it was (25-125)  µg/ spot. Then plate was developed in mobile phase and was developed to scan as mention above at 575 nm. Calibration curve here made was peak area v/s concentration of constituents. Accuracy (recovery) For UV-visible spectrophotometer solution of standard RES was added to previously analyzed sample solution at three different levels (80%, 100 % and 120%). Same procedure been followed to have a GYM accuracy by adding standard stock solution at three different levels (80%, 100 % and 120%). Amount of standard RES added was (8, 10 and 12  µg/ ml) to 10  µg/ ml sample solution. Amount of standard GYM added was (40, 50 and 60  µg/ ml) to 50  µg/ ml sample solution. For HPTLC known amount standard solution of RES (8, 10 12  µg/ ml) and GYM (40, 50 60  µg/ ml) added to previously analyzed sample solution having concentration of RES 10  µg/ spot and GYM 50  µg/ spot. Precision The intra-day and inter-day precision of proposed methods were determined by estimating corresponding responses three times on the same day and on three different days for three different concentrations. For UV-Visible spectroscopy RES concentrations were 8, 10 and 12  µg/ ml measured at wavelengths 318.4 nm and 349 nm.GYM concentrations were 45, 50 and 60  µg/ ml measured at wavelengths 303 nm and 349 nm. For HPTLC three different dilutions were made having both RES and GYM in those solutions ranging (RES 9, 10 and 12.5  µg/spot) and GYM (45, 50 and 62.5  µg/ spot). For repeatability in HPTLC, sample solution containing 10  µg/spot RES and 50  µg/ spot GYM was measured in terms of response. LOD LOQ The sensitivity of analytical method was evaluated by determining LOD and LOQ. They are measured by following equations: LOD: 3.3 à ¯Ã‚ Ã‚ ³/ S LOQ: 10 à ¯Ã‚ Ã‚ ³Ãƒ ¯Ã¢â€š ¬Ã‚ ¯Ãƒ ¯Ã¢â€š ¬Ã‚  S Here, à ¯Ã‚ Ã‚ ³ is standard deviation of intercept and S is slope in linearity equation. Specificity For HPTLC spots were scanned for its purity with standard sample and checked whether they give a same response or not. This was done by spectral scanning in WinCats HPTLC. Robustness The robustness of methods was studied by analyzing the same samples of RES and GYM with deliberate change in parameters. The changes in responses were noted. For HPTLC, spots scanned at ( ± 2 nm) and mobile phase ratio change was performed. For UV-Visible method solutions were scanned at ( ± 2 nm). 3. Results and Discussions Simultaneous estimation of RES and GYM was difficult task because they are isolated from herbal source and they have RES: GYM ratio 1:5 in marketed formulations. System suitability parameters System suitability run for HPTLC was performed before each validation run. Five replicate spots were made. Parameters monitored were Rf value and Peak areas of them. (Table 2) Table 2: System suitability Parameters HPTLC Optimization of Method For HPTLC Various experimental conditions such as the mobile phase and the wavelength of detection were optimized to achieve accurate, precise and reproducible results for the estimation of RES and GYM. Good resolution and sharp peaks with minimum tailing of these drugs (Rf RES 0.78, Rf GYM 0.236) was obtained by using mobile phase Chloroform: Methanol : Glacial acetic acid (13: 4 :0.5%) at wavelength of detection 575 nm. Figure 3 : optimized Chromatogram of HPTLC, RES (10  µg/spot) GYM ( 50  µg/spot) Figure 4: Wavelength selection for HPTLC of RES and GYM For UV-Visible Spectrophotometric Form overlain spectra (Figure 5) of methanolic solution of RES and GYM three wavelengths were finalized for analysis 303 nm, 318.4 nm and 349 nm. The method here used for simultaneous estimation is Q ratio method. Here both of constituents are measured at 349 nm isoabsorptive point and 303 nm and 318.4 nm GYM and RES respectively. Figure 5: wavelength selection after derivatization of GYM, BCL (Benzoyl Chloride) and RES Method validation of proposed methods Optimized methods were validated in compliance with ICH guidelines. The results of various parameters are discussed following: Linearity For UV Spectrophotometric method, linear correlation was obtained between absorbance and concentration for RES 5-25  µg/ ml at 318.4 nm 349 nm and GYM 25-125  µg/ ml 303 nm 349nm.( Table 3) For HPTLC method, linear correlations were obtained between peak area and concentration of RES was 5-25  µg/spot and GYM was 25- 125 µg/spot. (Table 4) Accuracy The percentage recovery values of RES and Gym were obtained in the range of 98% to 103 %, and relative standard deviation values for both constituents in two methods were less then 2%, it shows that methods are accurate for both constituents. Values are shown in table 3 and 4. Precision Inter-day and intra-day variation in quantification of RES and GYM showed that RSD values were always less than 2% during the analysis by both methods. These low RSD values show that methods are precise. Values of precision studies for UV spectrometry and HPTLC are in table 3 and 4 respectively. LOD and LOQ For UV-Visible spectrometry method LOD and LOQ for RES was found to be 0.09 µg/ml and 0.28 µg/ml respectively. LOD and LOQ for GYM were 0.63 µg/ml and 1.92 µg/ml respectively. For HPTLC method LOD and LOQ for RES were 0.065  µg/spot and 0.20  µg/ spot respectively. LOD and LOQ for GYM were 1.2  µg/spot and 3.87  µg/spot respectively. Specificity For HPTLC method, a good correlation was obtained between standard and sample spectra of RES and GYM correlation suggests that there in no interference in quantification of RES and GYM. Robustness Robustness of the methods was studied by performing assays of RES and GYM in capsule formulation. The parameters are deliberately altered and changes were recorded. Assay values were calculated in the changed parameters. Methods proved to be robust, because assay values in changed parameters were within limits. Assay of marketed formulation Assay of Resveratrol plus from ZENITH nutrition was performed in both the methods. Results of assay were compared with corresponding amounts claimed on capsule. The assay results are shown in table 3 4. Table 3: UV-Visible method Validation parameters Table 4: HPTLC Validation Parameters Conclusion Developed HPTLC and UV-Visible Spectrophotometric method was found to be simple, accurate, precise, rapid, sensitive and robust for the estimation of RES and GYM in combined dosage form. The validation data and recovery shows that methods are free from inferences of excipients used in formulations. Thus method is useful for both constituents to be estimated by both methods. References x

Friday, January 17, 2020

Project Metrics

â€Å"Metrics† is a term used to describe the measurement of a particular phenomenon. Project metrics therefore refers to the key indicators of what exactly has been done or achieved in a certain project. The objective of this is to be able to improve on the processes involved in the project performance. Project metrics thus is a system set in place to evaluate the project process employed in the attainment of results with an aim of improving such processes. They usually involve collecting and availing information regarding the status of the project.It is thus an important factor in project risk management as a review tool. One example of these metrics is the cost. Right before initiating a project, its financial aspect is normally catered for using budgetary control tools. Indeed, the economic viability of a project is a priority regardless of the final results expected of such a project. In this respect therefore, there are certain operations that should be conducted in the process of the project to monitor the cost element.The actual budget will thus be reviewed in light of the original budget. This yields certain variances whose magnitude can thus be reviewed to improve on the process. Quality is another key aspect in a project that would form the basis of metrics. Quality control is thus established to be able to measure the output of a particular process in light of a set standard. Defects in the system are identified and when adequately documented, these provide good grounds for review of the project process with an aim of improvement of the same.This is because in a business environment, quality compromise yields an adverse effect that translates to loss of economic gain which would otherwise be secured with the right standards of quality. In summary it can be said that in project management, the role of project metrics is extremely important and cannot be ignored. They constantly provide information, which when analyzed by the management is usef ul for decision making and the success of projects.

Thursday, January 9, 2020

The, Medicine Man, By Dr. Campbell - 854 Words

Movies are a source of entertainment across the world with multiple genres. What makes movies appealing to some viewers is the portrayal of accurate events in history or current events. While watching the movie â€Å"Medicine Man,† I have interpreted accurate evidence that is shown throughout the movie. One of the accurate portrayals in the movie was how the directors utilized the field of anthropology. Cultural relativism, which is the idea to not judge another culture with the beliefs of your own culture, was a major theme in the â€Å"Medicine Man.† This was conveyed through Dr. Campbell who lived with this native group for a time and instead of making judgements towards this unique and dissimilar group, he accepted them for who there are. Althought his research for curing cancer was why he was there, he did not dedicate his whole time to his research. Dr. Campbell learned the natives language and interacted with them on a daily bases. He also used his biological knowledge to cure some of the sickness that was brought into the village. This led for the people to call him the â€Å"Medicine Man.† Due to his altruistic actions, the people accepted Dr. Campbell and looked at him as a friend. Another man who used cultural relativism was Napoleon Chagnon, who did a case study in Brazil and Venezuela on the tribal group, the YÄ…nomamà ¶. He had a challenging start when he first stepped into the tropical forest that the natives inhabit but over time that changed. In the beginning the YÄ…nomamà ¶Show MoreRelatedThe Effects Of Medical Research On Professional Sports2097 Words   |  9 PagesCampbell 1 Brian Campbell Ms. Vyse English II Honors 24 March 2016 The Effect of Medical Research on Professional Sports in Concussion Football fanatics across the world live for the huge jarring hits that leave players laying on the field in shock. 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Wednesday, January 1, 2020

Effects Of War Being Touched By War - 828 Words

Christina Randazzo Mrs. Grabo Freshman English 12-10-2015 The Effects of War Being touched by war can change a person, especially if they’re someone like Ishmael Beah, the author of A Long Way Gone. Ishmael’s life started off as normally as yours or mine. He had a father, a mother, two brothers, a good group of friends, and a love for rap music. These were the days before the war. After the war came, everything changed, and now I feel that the phrase â€Å"A long way gone† applies to his life in many ways, whether it be physically, emotionally, or socially. Ishmael has gone through many physical changes throughout his time as a boy soldier. When he was a boy, he had never even touched drugs, but once he was plunged into the heart of the war, drugs became a part of the everyday routine. The drugs that they gave him to keep him awake and energized did their job. They did it a little too well. He is so full of drugs that he hasn’t slept or eaten for weeks. 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