{"id":4622,"date":"2014-11-14T10:41:34","date_gmt":"2014-11-14T03:41:34","guid":{"rendered":"http:\/\/swallow-nest.com\/article\/2014\/11\/14\/the-detection-of-staphylococcus-aureus-in-swiftlets-nest-using-immunohistochemistry-streptavidin-biotin\/"},"modified":"2014-11-14T10:41:34","modified_gmt":"2014-11-14T03:41:34","slug":"the-detection-of-staphylococcus-aureus-in-swiftlets-nest-using-immunohistochemistry-streptavidin-biotin-2","status":"publish","type":"post","link":"https:\/\/indonesia-product.com\/news\/the-detection-of-staphylococcus-aureus-in-swiftlets-nest-using-immunohistochemistry-streptavidin-biotin-2\/","title":{"rendered":"THE DETECTION OF Staphylococcus aureus IN SWIFTLETS&#039; NEST   USING IMMUNOHISTOCHEMISTRY (STREPTAVIDIN BIOTIN)"},"content":{"rendered":"<p><!--adsense--><\/p>\n<p>.journal.unair.ac.id<br \/>\nRetno Oktorina*, Soedarmanto Indarjulianto**, Sitarina Widyarini**, Hastari Wuryastuti**, R. Wasito**      ABSTRACT    A study to detect the presence of Staphylococcus aureus in swiftlets&#8217; nest using immunohistochemistry (Streptavidin  biotin Complex) has been successfully done.<br \/>\n<!--more--><br \/>\n Tissue and supernatant were made from the nest, and the presence of the  bacteria Staphylococcus aureus was detected by means of immunohistochemical method. As positive control, we used  Staphylococcus aureus culture, while for negative control we replaced Staphylococcus aureus monoclonal antibody  with Phospat Buffer Saline (PBS). The result showed that staining with Staphylococcus aureus monoclonal antibody in  swiftlets&#8217; nest tissue revealed the presence of Staphylococcus aureus as a brownish group or cluster, resulting from the  reaction of enzymes and chromogen in Streptavidin Biotin Complex. Based on this study, it can be concluded that  immunohistochemical method (Streptavidin Biotin Complex) can be used to detect the presence of Staphylococcus  aureus in swiftlets&#8217; nest.    Keywords: swiftlets&#8217; nest, S. aureus, immunohistochemistry<\/p>\n<p>INTRODUCTION    A major challenge for Indonesia is to produce animal  food products which are safe for consumers&#8217; health.  Animal food safety is not only the world&#8217;s issue  (Anonym, 2000), but also every indivual&#8217;s concern. It is  a consumer&#8217;s right to have safe animal food. Indonesia is  the largest producer and supplier of swiftlets&#8217; nest, with  Hongkong, USA, Singapore, Malaysia, China, Japan,  and UK as the major export destinations (Iswonto,  2002). Playing the role as largest producer, Indonesia  should maintain the aspect of food quality as the main  consideration in trade. Market requirement and product  suitability for consumers should be met by increasing  product acceptability and competitiveness in global  market (Anonym, 2000).    Swiftlets&#8217; nest is an exotic or delicate food. In addition  as a delicious serving, it can also be used as material for  medications that improves physical strength (Winarno,  1994; Budiman, 2002; Iswanto, 2002). As in other food  materials, swiftlets&#8217; nest may subject to damage  resulting from pesticide residuals, animal drugs, heavy  metals, other contaminants, as well as the growth of  microbes, such as bacteria, virus, yeast, and fungi,  which may cause food-borne disease.    To support the availability of safe food products as the  basic consideration in trade, we need microbial  detection method for swiftlets&#8217; nest. In a preliminary     study, Animal Quarantine Board (Balai Karantina  Hewan) in cooperation with Airlangga University  School of Pharmacy had undergone a test on  Microbiological Quality Control for export swiftlets&#8217;  nest in Animal Quarantine Juanda (unpublished data).  The result of this preliminary study, obtained using  rapid test (Oxoid, United Kingdom) and followed with  fertilization in agar media, showed that Staphylococcus  spp was identified in five samples of swiftlets&#8217; nest,  while Escherichia coli was identified in one sample.  Salmonella spp and Pseudomonas spp were not found.    Staphylococcus spp is a group of bacteria that plays an  important role in food microbiology, and  Staphylococcus aureus is the prominent bacteria in food  because during its growth the organism can produce  enterotoxin. Ecologically, Staphylococcus aureus is  closely related with human beings. In largest amount of  cooked or salted foods, Staphylococcus aureus can  unceasingly grow until reaching a hazardous level  (Buckle, 1987). Based on this preliminary study, a fast  and accurate method to detect Staphylococcus aureus in  swiftlets&#8217; nest was needed. The method that is recently  developing is the use of immunohistochemistry by  means of the principle of specific binding between  antigen and antibody which was visualized through  enzymes and substrates. This method used basic  principles of immunology in tissue or cells.<\/p>\n<p>MATERIALS AND METHODS<\/p>\n<p>This study used swiftlets&#8217; nest samples ready to be  exported through Juanda Airport. The samples were  processed to make preparations in Veterinary Disease  Inspection Bureau (Balai Penyidikan Penyakit  Veteriner, BPPV) Regional IV Yogyakarta in  accordance with standard procedure of BPPV  laboratory. The swiftlets&#8217; nest preparation in paraffin  embedded tissue section was put onto Poly-L-lysin  (SIGMA)-coated glass object. The  immunohistochemical staining used Streptavidin Biotin,  with stages as recommended by Wasito (1997). The  swiftlets&#8217; nest preparation was paraffinized by giving (a)  xylene, three times each for 2 minutes, (b) 100%  ethanol, twice each for 2 minutes, (c) 95% ethanol, once  each for 2 minutes, (d) 50% ethanol, each for 2 minutes,  and (e) distilled water, twice each for 2 minutes, and  Phosphate Buffer Saline (PBS) of 0.01 m with pH 7.1  for 5 &#8211; 10 minutes. Subsequently, the preparation was  immersed in H2O2 to remove endogeneous peroxidase,  and incubated in a microwave. The preparation was then  washed with PBS for 10 minutes, and incubated with  blocking serum (V Block) solution for 10 minutes. The  excessive serum was removed from the preparation and  the latter was directly given with primer antibody, i.e.  Staphylococcus aureus monoclonal antibody and  incubated at room temperature for 45 minutes, and  washed with PBS for 10 minutes. Antigen retrieval was  done using citric acid and microwaved for 10 minutes  (Shan et al, 1997). The preparation was incubated with  Biotynilated Secondary Antibody (Lab Vision, USA) at  room temperature for 10 minutes, incubated with  chromogen substrate (Lab Vision, USA) at room  temperature for 15 minutes, washed with distilled water,  and mounted with glycerol to be observed under the  microscope.    For culture preparation of the isolates of Staphylococcus  aureus and supernatant from swiftlets&#8217; nest sample, the  stages of immunohistochemical staining were the same  as those in paraffin-embedded tissue section. The  difference was that in supernatant preparation, the  swiftlets&#8217; nest should be paraffinized and washed  directly for 5 minutes, while the rest of the procedures  were all the same. To obtain supernatant preparation, 5  grams of swiftlets&#8217; nest sample were finely ground,  added with physiologic NaCl and left overnight.  Subsequently, the preparation was dripped on Poli-Llysine-coated glass object, and incubated in microwave  for 12 hours and subjected to immunohistochemical  staining using Streptavidin Biotin method (Wasito,  1997). As positive control for this staining method, we  used Staphylococcus aureus colony. Negative control  was made by replacing primary antibody with  Phosphate Buffer Saline (PBS).<\/p>\n<p>  RESULTS AND DISCUSSION<br \/>\n The objective of this study was to apply  immunohistochemical method by using Streptavidin  Biotin Complex. This technique is a modification of  indirect method, in which one antigen from swiftlets&#8217;  nest is bound by antibody in two stages. First, the  primary antibody is directly bound to antigen.  Afterwards, the antibody will be bound to biotinilyzedprimary antibody. The binding between antigen and  antibody would be visualized by the change of enzymes  and substrates into brownish color (Hoffman, 1996;  Wasito, 1997; Harkow F and Lane, 1999). The  application of immunohistochemical method is  immunohistochemical staining to culture, supernatant,  and swiftlets&#8217; net tissue. Immunohistochemically-stained  Staphylococcus aureus culture from the nest revealed  brown precipitation, indicating the binding between  antigen and antibody as visualized through the reaction  of peroxidase and 3,3 diaminobenzidine  tetrahydrochloride (Figure 1). The Staphylococcus  aureus looks grouped or clustered.    Immunohistochemically-stained swiftlets&#8217; nest  supernatant showed the presence of antigen  (Staphylococcus aureus) and antibody binding, which  was visualized by the presence of brown precipitation  (Figure 2). This was in line with the basic principle of  chromogen, a marker that can visualize marker  substance at immunocomplex binding in  immunohistochemical staining. In this principle, the  binding between chromogen and peroxide (marker  substance) is visualized brown by using 3,3  diamonobenzidine tetrahydrochloride chromogen  (Baroff and Cook, 1994; Wasito, 1997). The paraffin  embedded tissue section of swiftlets&#8217; nest using  Streptavidin Biotin method (Lab Vision, USA) showed  the result of antigen (Staphylococcus aureus) and  antibody binding visualized as having brown color  (Figure 3).<\/p>\n<p>Those results showed that immunohistochemical  method using Streptavidin Biotin can be used to detect  Staphylococcus aureus in supernatant and swiftlets&#8217; nest  tissue. Previous studies were reported by Cleary et al  (2004), Priambodo (2004) and Tsusumi et al (1991)  who detected bacteria in intestinal epithelium, blood and  urine using immunohistochemical staining. In these  studies the bacteria was apparent in the form of cluster  or clump (bacterial coated antibody).    In culture preparation using immunohistochemical  staining (Streptavidin biotin), the supernatant and  preparation from swiftlets&#8217; nest tissue had a brown  color, a result of binding between antigen  (Staphylococcus aureus) and its monoclonal antibody  which was visualized through chromogen substrate in  the colony of the bacteria that formed a group or cluster  (Duguid, 1989).      CONCLUSION    Immunohistochemical staining can be used to detect the  presence of Staphylococcus aureus in swiftlet&#8217;s nest.      REFERENCES    Anonim, 2000. Petunjuk Teknis Operasional Tindak  Karantina Hewan Untuk Sarang Burung Walet,  Penerbit Proyek Pusat Karantina, Pertanian, Jakarta  Bbckle KA, Edwards RA, Fleet, Wooton M, 1978. Food  Science, translated by Hari Purnomo dan Adiono,  Penerbit Universitas Indonesia  Budiman A, 2002. Memproduksi Sarang Walet Kualitas  Atas, PT. Penebar Swadaya, jakarta    Bancroft JD and Cook HC, 1994. Manual of  histological techniques and their diagnostic  application. Churchill Livingstone, United Kingdom.  Cleary J, Ching Lai L, Robert KS, Stratman IA,  Donnenberg MS, Frankel G, Knutton S, 2004.  Enteropathogenic Esherichia Coli (EPEC) adhesion to  intestinal epithelial cells; role of bundle formingpili  (BFP), Esp A flamens and intimin. J Microbiology  150, pp. 527-538.  Duguid JP, 1989. Staphylococcus: Cluster Farming  Gram Positive Cocci. In: Collee, JG, Duguid JP,  Frasser and Marmion BP. Pratical Medical  Microbiology, 13th ed. Churchill Livingstone,  Edinburgh, London, Melbourne, New York, pp. 305308.  Harlow E and Lane, 1999. Using Antibodies, A  Laboratory Manual Cold Spring Harbour Laboratory  Press, New York.  Hofman F, 1996. Immunohistochemistry. In: Current  Protocols in Immunology, John Wiley and sons, Inc.  pp. 5.8.1-5.8.23.  Iswanto H, 2002. Kiat Mengatasi Permasalahan Praktis  Walet,  PT Agromedia Pustaka, pp. 41-50.  Priyambodo Y, 2001. Deteksi bakteri Berselubung  Antibodi Dalam Sedimen Air Kemih Dengan Uji  Streptavidin Biotin, Dissertasion, Airlangga  University, Surabaya.  Tsutsumi Y, Kawai K, Nagakura K, 1991. Use of  patients sera for immunoperoxidase demonstration of  infection agents paraffin sections. J Acta Pathol  Japan 41 (9), pp. 673-679.  Wasito, R, 1997 Immunocytochemistry. In: Diagnostic  Pathology : Use of Immunohistochemocal Tecniques  For Detecting Porcine Specific RNA Transmisible  Gastroenteritisvicus In Vivo. Indon. J. Biotech 6, pp.  121-124.  Winarno, 1994. Sarang Burung Walet, Bahan Hidangan  Eksotis, Bonus Femina (3): 22, Jakarta.      <\/p>\n","protected":false},"excerpt":{"rendered":"<p>.journal.unair.ac.id Retno Oktorina*, Soedarmanto Indarjulianto**, Sitarina Widyarini**, Hastari Wuryastuti**, R. Wasito** ABSTRACT A study to detect the presence of Staphylococcus aureus in swiftlets&#8217; nest using immunohistochemistry (Streptavidin biotin Complex) has been successfully done.<\/p>\n","protected":false},"author":1,"featured_media":0,"comment_status":"open","ping_status":"open","sticky":false,"template":"","format":"standard","meta":[],"categories":[413],"tags":[],"yoast_head":"<!-- This site is optimized with the Yoast SEO plugin v19.6 - https:\/\/yoast.com\/wordpress\/plugins\/seo\/ -->\n<title>THE DETECTION OF Staphylococcus aureus IN SWIFTLETS&#039; NEST  USING IMMUNOHISTOCHEMISTRY (STREPTAVIDIN BIOTIN) - Directory of wholesale, manufacturers, distributors, importer and exporter in Indonesia<\/title>\n<meta name=\"robots\" content=\"index, follow, max-snippet:-1, max-image-preview:large, max-video-preview:-1\" \/>\n<link rel=\"canonical\" href=\"https:\/\/indonesia-product.com\/news\/the-detection-of-staphylococcus-aureus-in-swiftlets-nest-using-immunohistochemistry-streptavidin-biotin-2\/\" \/>\n<meta property=\"og:locale\" content=\"en_US\" \/>\n<meta property=\"og:type\" content=\"article\" \/>\n<meta property=\"og:title\" content=\"THE DETECTION OF Staphylococcus aureus IN SWIFTLETS&#039; NEST  USING IMMUNOHISTOCHEMISTRY (STREPTAVIDIN BIOTIN) - Directory of wholesale, manufacturers, distributors, importer and exporter in Indonesia\" \/>\n<meta property=\"og:description\" content=\".journal.unair.ac.id Retno Oktorina*, Soedarmanto Indarjulianto**, Sitarina Widyarini**, Hastari Wuryastuti**, R. 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