The reagent has a dark orange colour and is stable for several days in room temperature. [Crossref]. Our developments initially aimed the monitoring of the effect of ultrasound (US) in the activity of these two enzymes [7,8], and sought the improvement / addition of methodological features that lead to complementary information (glucose yield) about amyloglucosidase using a similar experimental protocol. The values in parentheses are the limits of the 95% confidence levels intervals, and starch mass is expressed in mg. Here we introduced an improved method capable to measure the activity of alpha-amylase and amyloglucosidase from different sources based on a quantitative starch-iodine assay. Transfer 50L of sample supernatant (or standard), and add 150L of GOPOD reagent to each well of the microplate. Microbiol Res 207:116133, Srinivas A, Rahul K, Sasikala C, Subhash Y, Ramaprasad EVV, Ramana CV (2012) Georgenia satyanarayanai sp. Otherwise, the extract from Chrysactinia mexicana had an IC50 value of 9.09 g mL-1, indicating that the extract from this plant also contained bioactive metabolites, which have an inhibitory effect on the enzyme -amylase. <>/ExtGState<>/XObject<>/ProcSet[/PDF/Text/ImageB/ImageC/ImageI] >>/MediaBox[ 0 0 595.32 841.92] /Contents 4 0 R/Group<>/Tabs/S/StructParents 0>> Spectrosc. Xiao et al. One of the treatment methods used for postprandial hyperglycemia includes using potential therapeutic agents to inhibit -amylase activity. Production of Actinobacteria Amylase by Fermentation in Solid State Using Residues of Licuri Palm (Syagrus coronata). One hundred twenty five patients were included in the present study. 2012, 13, 427. An illustrative linear (R2=0.999) calibration curve is abs580nm=0.061 (0.025)+0.366 (0.014) mstarch. The xylanase was immobilized for 4 h on 10 BCL aldehydeagarose gel by multicovalent attachment in 100 mM bicarbonate buffer at 25 C and pH 10 (Guisan, 1988).Periodically, the Soluble starch (PN: S9765), starch from corn (PN: S4126), starch from potato (PN: S4251), starch from rice (PN: S7260), starch from wheat (PN: S5127, unmodified), I2 (PN: 207772, 99.8%), 85% (w/w) o-phosphoric acid (PN: 79620), and acetic acid (PN: 695092, 99.7%) were purchased from Sigma-Aldrich (St. Louis, MO, USA). 2020-04-29T17:28:43+05:302017-05-24T07:28:08ZMicrosoft Office Word 2007 Biol Control 109:113, Shukla RJ, Singh SP (2015) Characteristics and thermodynamics of -amylase from thermophilic actinobacterium, Laceyellasacchari TSI-2R. Changes in conditions/parameters, such as enzyme concentrations (< 0.15 U mL 11 Bhat, M.; Zinjarde, S. S.; Bhargava, S. Y.; Kumar, A. R.; Joshi, B. N.; J. Evidence-Based Complementary Altern. sharing sensitive information, make sure youre on a federal In this experiment, acarbose at a concentration of 1.05 g mL-1 was used to record the desired maximum signal. The In this experiment, acarbose at a concentration of 5 g mL-1 was used to record the desired minimum signal. Anal. This protocol helps you to understand the applications of amylase enzyme. Biochem. Simultaneously setup the color developed at 520nm. 2 0 obj These findings demonstrated that our optimized and validated method is highly selective, enabling the identification of samples with or without potent activity. 8600 Rockville Pike Disclaimer, National Library of Medicine [Crossref]-1616 United States Pharmacopeial Convention; The United States pharmacopeia: the national formulary; Rockville, Md., United States pharmacopeial convention, 1980.,2727 Iversen, P.; Beck, B.; Chen, Y.; Dere, W.; Devanarayan, V.; Eastwood, B. J.; Farmen, M. W.; Iturria, S. J.; Montrose, C.; Moore, R. A.; Weidner, J. R.; Sittampalam, G. S. In HTS Assay Validation; Markossian, S.; Grossman, A.; Brimacombe, K.; Arkin, M.; Auld, D.; Austin, C. P.; Baell, J.; Chung, T. D. Y.; Coussens, N. P.; Dahlin, J. L.; Devanarayan, V.; Foley, T. L.; Glicksman, M.; Hall, M. D.; Haas, J. V.; Hoare, S. R. J.; Inglese, J.; Iversen, P. W.; Kales, S. C.; Lal-Nag, M.; Li, Z.; McGee, J.; McManus, O.; Riss, T.; Saradjian, P.; Sittampalam, G. S.; Tarselli, M.; Trask, O. J.; Wang, Y.; Weidner, J. R.; Wildey, M. J.; Wilson, K.; Xia, M.; Xu, X., eds. After preincubation, 100 L of starch was added (final concentration 0.38 mg mL-1) and incubated at 37 C for 5.5 min for enzymatic action. Lilly (2007) recommended the use of the substrate at or below the Km value. Pharmacol. Bookshelf We adopted this strategy to separate the solid particles that remained after the hydrolysis of different pure starches mediated by amyloglucosidase (glucose yield protocol, step 5). 2018, 14, 458. Unit of Microbiology, Department of Biology, University of Patras, http://www.microbiology.biology.upatras.gr. From a quantitative point of view, the determination of amylase activity is generally carried out by a spectrophotometric method using DNS (3,5-dinitosalicylic acid) in a colorimetric reaction with reducing sugars released as a result of the hydrolysis of starch, although other colorimetric methodologies are possible [ 1, 3, 4, 5, 6 ]. The use of soluble starch also allowed the standardization of the working conditions, avoiding any influence of the solubility of the starch in the final result. Without salivary amylase, we would not be able to digest carbohydrates properly and would not get the total nutritional value from these foods. 2019 Oct;18(4):2531-2539. doi: 10.3892/etm.2019.7840. Diabetes mellitus is a chronic metabolic disorder characterized by hyperglycemia (high blood sugar levels) due to insulin resistance or absolute lack of insulin production. Amylase, like other enzymes, works as a catalyst. This article will discuss the different applications of amylase. [Crossref]. Acarbose, an inhibitor of the amylase enzyme, was evaluated at six different concentration levels by regression analysis. Fig. It helps you protect your students from spelling mistakes and volumetric errors. Enzyme immobilization Preparation of alginate beads Alginate gel beads were prepared according to Awad et al. The most commonly used method to measure -amylase in wheat grain is the Hagburg Falling Number method but the values are also influenced by rheological properties of starch in the grain.1,2 The most specific method for the measurement of -amylase is the Ceralpha method which employs a defined substrate, 4,6-O-benzylidene--4-nitrophenyl- Comparison of such results will lead to low reliability of these in vitro methods. [Crossref] Although other protocols are based either on the glucose oxidase reaction or on the determination by fluorescence, they are commonly used in microplates. [Crossref] Hence, it is necessary to look for inhibitors of -amylase from natural sources with fewer side effects. Google Scholar, Vasconcelos NM, Pinto GAS, Arago FAS (2013) Boletim de Pesquisa n. 88, Determinao de Acares Redutores pelo cido 3,5-Dinitrosaliclico: Histrico do Desenvolvimento do Mtodo e Estabelecimento de um Protocolo para o Laboratrio de Bioprocessos. [Crossref], a determination coefficient of 0.9947, a slope of 11.493, and an IC50 value of 2.9 0.03 g mL-1 (data not shown). [Crossref], The phytochemical analysis indicated the presence of various metabolites such as alkaloids, flavonoids, terpenes, steroids, and phenols. [Crossref],33 Moein, S.; Pimoradloo, E.; Moein, M.; Vessal, M.; BioMed Res. To each tube, 100 L of plant extracts with different concentrations (final concentration 6 g mL-1 to 200 g mL-1) and 100 L of -amylase (final concentration 0.15 U mL-1 in phosphate buffer) were added and incubated at 37 C for 7.2 min. Biocatal Agric Biotechnol 23:101452, Thampi A, Bhai RS (2017) Rhizosphere actinobacteria for combating Phytophthora capsici and Sclerotium rolfsii, the major soil borne pathogens of black pepper (Piper nigrum L.). Then, we have partially purified these amylases employing three conventional methods: (a) cold acetone precipitation, (b) ion-exchange chromatography, and (c) gel filtration chromatography. The use of phosphate buffer also affected the response. In the present method of Millers reaction, the product to be analyzed was obtained by heating it in a boiling water bath. This method intends to facilitate the implementation of a new routine determination of alpha-amylase and amyloglucosidase activities in any laboratory that could deal with amylolytic enzymes by providing all the necessary experimental details and conditions that could maximize the performance of the method. [Crossref]. Ten different experiments were performed. R. P.; Mol. The error percentage was calculated to be 5.46%, which indicates that the method is accurate. Bethesda, MD 20894, Web Policies It was initially termed In these experimental conditions, an illustrative calibration curve is abs505nm=0.042 (0.005)+0.0846 (0.0008) mglucose. Home - Protocols - Quantitative Analysis - Assay of Salivary Amylase enzyme activity. Set up the standards of different test tubes and repeat the experiment as per the test and measure the color developed at 520nm absorbance. 2023 Springer Nature Switzerland AG. Max signal: The maximum absorbance was recorded by the assay procedure. 14 Food and Drug Administration (USA); Bioanalytical method validation guidance for industry, US Department of Health and Human Services Food and Drug Administration Center for Drug Evaluation and Research and Center for Veterinary Medicine, 2018, available at https://www.fda.gov/files/drugs/published/Bioanalytical-Method-Validation-Guidance-for-Industry.pdf, accessed June 2022. Additionally, the significant factors were optimized using the rules of the basic sequential simplex method and the combination of conditions that maximized the inhibition percentage with the lowest photometric error. The ethanol extract of A. Maxicana L. leaves possessed Multi-Mechanistic In Vitro Evaluation of Antihyperglycemic, Antioxidant and Antiglycation Activities of Three Phenolic-Rich Indian Red Rice Genotypes and In Silico Evaluation of Their Phenolic Metabolites. Gangadharan D., Sivaramakrishnan S. Amylolytic enzymes. The characterization of both assays for the evaluation of the activity of amylolytic enzymes and glucose yield considered its linear range, sensitivity, repeatability, and limit of detection (LOD). J. It is defined as the combinatorial effect of all components of the analysis other than the analyte that is to be measured.2828 McNaught, A. D.; Wilkinson, A.; Compendium of Chemical Terminology (IUPAC Chemical Data), 2nd ed., Wiley: New Jersey, 1997. Hence, a reliable protocol for preparing the starch solution is an important aspect regarding the need for a batch to batch reproducibility. amylase, any member of a class of enzymes that catalyze the hydrolysis (splitting of a compound by addition of a water molecule) of starch into smaller carbohydrate molecules such as maltose (a molecule composed of two glucose molecules). Analysis - assay of salivary amylase, we would not get the total nutritional value from these foods of! 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