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  • #16
    الأخ بدرين المحترم
    السلام عليكم
    كيف يمكن تحميل الكتاب, اين الرابط

    تعليق


    • #17
      حقيقة لدي كتاب وحاولت تحميلة عبر الايقونات الظاهرة علي الرد السريع ولكني فشلت

      تعليق


      • #18
        السلام عليكم أخي فارس
        انا دكتور في الجامعة واقوم ببحث مع الطلاب في مجال تحليل المياه العذبة وآمل في الاستفادة من خبرتك حول افضل طريقة لتحليل ميكروبات المياه العذبة
        أخوك ناجي

        تعليق


        • #19
          البكتيريا والفطريات وكذلك البروتوزوا ان امكن

          تعليق


          • #20
            المشاركة الأصلية بواسطة ناجي التومي مشاهدة المشاركة
            البكتيريا والفطريات وكذلك البروتوزوا ان امكن







            *




            LEARNING OBJECTIVES




            After completing this practical you will be able to:
            1- Know various methods used for testing potable water.
            2- Test the quality of the potable water for drinking.




            INTRODUCTION




            Drinking water is acceptable and fit for drinking when it is clear, colourless, odourless and without disagreeable taste. Microscopically it should be free from pathogenic organisms.
            Natural sources of water usually contain some saprophytic bacteria, such as Pseudomonas, Serratia, Flavobacterium, Chromobacterium, Acinetobacter, Alcaligenes, etc. These saprophytes are harmless.Water gets contaminated by pathogens which are introduced into water by sewage pollution. A wide varieties of diseases are transmitted by contaminated water. There are some indicator organisms, whose presence indicates the contamination of water with fecal matter. These are:
            1 Coliforms.
            2 Fecal (thermotolerant) coliforms.
            3 Faecal Escherichia coli.
            4 Faecal Streptococci, and
            5 Clostridium perfringens.




            Coliforms
            Coliforms are defined as members of the family Enterobacteriaeceae which grow in the presence of bile salts and produce acid and gas from lactose within 48 hours at 37°C. In order to include anaerogenic bacteria and those which are nonlactose fermenters, it has been modified as the members of the Enterobacteriaeceae capable of growing galactosidase at 37°C that normally posses.The total coliform count is widely regarded as the most reliable indicator of potable water quality. However, the presence of coliforms not necessarily indicate faecal or sewage contamination, because, these organisms are present in large quantities in the environment.




            Faecal or thermotolerant coliforms
            These satisfy the criteria for coliforms but have the additional property of the ability to grow at a higher temperature 44°C.




            Faecal Escherichia coli
            These are defined as thermotolerant coliforms which ferment lactose (or) mannitol at 44°C with the production of acid and gas within 24 hours and also form indole from tryptophan at 44°C. The presence of E. coli is considered as the contamination of water with feces of human or animal origin.
            Faecal streptococci
            These are catalase negative, Gram positive cocci present in the intestinal tract of man and animals. These organisms have the Lancefield group D antigen, hydrolyse aesculin and can grow at 45°C, in the presence of azide and 40% bile. Such organisms which can survive 60°C for 30 min and can grow at 10°C at pH 9.6 and in 6.5% of sodium chloride (NaCl) belong to the genus Enterococcus (Enterococcus faecalis and E. faecium) .




            Clostridium perfringens
            The presence of this organism in water in the absence of other indicators of contamination of water implies remote or intermittent fecal pollution. Viruses in water are destroyed by chlorination. When the concentration of free residual chlorine is at least 0.5 mg per litre, for a minimum contact period of 30 minutes at pH below 8 and a turbidity of 1 nephelometric turbidity unit or less, protozoa such as Entamoeba histolytica, Giardia species and Balantidium coli may be present in the drinking water. Coliforms are not the reliable indicator of protozoal contamination.




            Collection of water samples
            Water is collected in heat sterilised bottles containing a sufficient volume of sodium thiosulphate to neutralise the bactericidal effect of any chlorine or chloramine in the water. For collection from tap, water is allowed to run to waste for 2–3 min. before collecting it into the bottle. When collecting water samples from lakes or streams the bottle is opened at a depth of about 30 cm with its mouth facing the current. At least 100 ml of water to be tested is collected in each bottle.
            After collecting the water in the bottle, the bottle is stoppered, and sent to the laboratory as quickly as possible within 6 hours keeping it in a cool container and protecting it from light.




            PRINCIPLE
            The following tests can be done for bacteriological analysis of water:
            1 Plate count.
            2 Detection of coliform bacteria and E. coli.
            a Presumptive coliform count: multiple tube technique.
            b Differential coliform test.
            c Membrane filtration method.
            3 Detection of faecal streptococci.
            4 Examination of Cl. perfringens, and
            5 Test for pathogenic bacteria.




            Plate count
            This consists of inoculating the nutrient agar with water to be tested and incubating the agar aerobically in parallel at 37°C for 1–2 days and at 22°C for 3 days. After incubation number of the colonies formed in the agar are counted. Those which grow at 37°C are associated with organic material of human or animal origin and those growing at a lower temperature are mainly saprophytes that normally inhabit water, soil, and vegetables. The agar count at 22°C gives an indication of the amount of decomposing organic matter in the water available for bacterial nutrition. Though these are non-pathogenic the greater the amount of organic matter present, the more likely is the water to be contaminated with parasitic and potentially pathogenic organisms.
            The agar count at 37°C is a more important index of dangerous pollution.
            Detection of coliform bacteria and E.coli
            Presumptive coliform test – Multiple tube
            technique
            The test is called presumptive, because of the presumption that the reactions are due to coliforms organisms. The count is made by adding varying quantities of water (0.1 ml–50 ml) to bile salt lactose peptone water with an indicator for acidity. Acid and gas formation indicate the growth of coliform bacilli.




            Differential coliform test
            This is called Eijkman test. This test is usually employed to find out whether the coliform bacilli detected in the presumptive test are E. coli or not. After the usual presumptive test, subcultures are made from all the bottles showing acid and gas to fresh tubes of single strength MacConkey medium already warmed to 37°C. They are incubated at 44°C for 24 hours. Those showing gas in Durham’s tubes contain E. coli. From the number of positive tubes obtained, results are read off the probability tables. Further confirmation of the presence of E. coli is done by testing for indole production and citrate utilization tests.




            Membrane filtration method
            A measured volume of water is filtered through a Millipore filter. All the bacteria present are retained on its surface. This is then placed on suitable media and incubated at the appropriate temperatures. Colonies on the surface of the membrane are counted. After 18 hours of incubation the presumptive coliform counts and detection of E. coli can be directly made.




            Detection of faecal streptococci
            Subcultures are made into tubes containing 5 ml of glucose azide broth from the positive bottles in the above test. Streptococcus faecalis if present produces acid in the medium within 18 hours at 45°C.




            Examination for Cl. perfringens
            Water is incubated in litmus milk medium at 37°C for 5 days, if positive, stormy fermentation occurs.




            Examination for pathognic bactrial cells test
            For other special pathogens like Salmonella, Vibrio, etc. corresponding special media are used.
            In this chapter Presumptive coliform test and differential coliform test will be discussed.




            REQUIREMENTS
            I -Equipments
            Bacteriological incubator, autoclave and water bath.




            II- Reagents
            MacConkey broth, brilliant green bile broth Preparation of MacConkey broth: This is prepared by mixing pancreatic digest of gelatin, 20 grams; lactose, 10 grams; bile salt, 5 grams; bromocresol purple, 0.01 grams and final pH (at 25°C) is adjusted at 7.3 ± 0.2.
            Preparation of double strength medium: It is prepared by suspending 35 grams in 500 ml of distilled water and heated to dissolve the medium completely. 50 ml and 10 ml of the media are dispensed into screw capped bottles with inverted Durham’s tubes and are sterilized by autoclaving at 15 lbs (121°C for 15 minutes).
            Preparation of single strength medium: It is prepared by suspending 3.5grams in 100 ml of distilled water. 5 ml quantities of the medium are dispensed in screw capped bottles with inverted Durham’s tubes and are sterilized by autoclaving at 15 lbs (121°C for 15 minutes).
            Preparation of brilliant green bile broth (BGBB): This is prepared by mixing peptic digest of animal tissue, 10 grams; lactose, 10 grams; ox gall, 20 grams and brilliant green, 0.0133 gm and adjusting the final pH (at 25°C) to 7.2 ± 0.2. 4 grams of the medium is suspended in 100 ml distilled water and mixed well. The media is distributed in 5ml volumes in test tubes with inverted Durham’s tubes and sterilized by autoclaving at 15 1bs pressure (121°C) for 15 minutes.




            III- Specimen
            Water specimen to be tested.




            PROCEDURE
            1- Collect 500 ml of water in a sterile bottle.
            2- Inoculate water sample immediately into the MacConkey broth medium.
            3- Inoculate 50 ml of water into 50 ml double strength media (1 bottle)
            4- Inoculate 10 ml of water into 10 ml double strength medium (5 bottles).
            5- Inoculate 1 ml of water into 5ml single strength medium (5 bottles).
            6- Incubate all the bottles at 37°C for 48 hours.
            7- Check for acid and gas after 24 hours and 48 hours.
            8 -Any positives are inoculated into brilliant green bile broth and peptone water.
            9 -Incubate at 44°C in a water bath overnight.




            QUALITY CONTROL
            Sterility of media and strength of media should be properly checked.




            OBSERVATIONS
            Observe for the presence of gas and production of indole. Presence of gas in brilliant green bile broth and indole production at 44°C is indicative of the presence of E. coli. For interpretation refer MacGrady’s table.




            RESULTS AND INTERPRETATION
            Presumptive coliform count The no. of bottles showing acid and gas is counted and compared with the MacGrady’s table. Result is expressed as- coliforms most probable no (MPN)/
            100ml. e.g. for Presumptive coliform count No. of tubes giving positive reaction 50 ml 10 ml 1 ml * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * *1 * * * *2 * * * 2
            Result: Coliforms most probable no 10/100 ml.
            Differential coliform count
            The no of tubes showing positive results i.e. both gas productions in BGBB and Indole test at 44°C is compared with MacGrady’s table. Result is expressed a Escherichia coli Most probable No (MPN) / 100 ml. Eg. for Differential coliform counts: No. of tubes giving positive reaction.
            50 ml * 10 ml * *1 ml
            1 * * * * * 1 * * * * *1
            Results: Escherichia coli MPN—— 5 /100 ml
            Report: Unsatisfactory.
            Grades of the quality of drinking water supplied as determined by results of periodic Escherichia coli and coliform counts is listed in the table 84-1.






            *
            *
            [/COLOR][/B]

            تعليق


            • #21
              المشاركة الأصلية بواسطة ناجي التومي مشاهدة المشاركة
              البكتيريا والفطريات وكذلك البروتوزوا ان امكن







              *




              [LEFT][RIGHT][LEFT]LEARNING OBJECTIVES




              After completing this practical you will be able to:
              1- Know various methods used for testing potable water.
              2- Test the quality of the potable water for drinking.




              INTRODUCTION




              Drinking water is acceptable and fit for drinking when it is clear, colourless, odourless and without disagreeable taste. Microscopically it should be free from pathogenic organisms.
              Natural sources of water usually contain some saprophytic bacteria, such as Pseudomonas, Serratia, Flavobacterium, Chromobacterium, Acinetobacter, Alcaligenes, etc. These saprophytes are harmless.Water gets contaminated by pathogens which are introduced into water by sewage pollution. A wide varieties of diseases are transmitted by contaminated water. There are some indicator organisms, whose presence indicates the contamination of water with fecal matter. These are:
              1 Coliforms.
              2 Fecal (thermotolerant) coliforms.
              3 Faecal Escherichia coli.
              4 Faecal Streptococci, and
              5 Clostridium perfringens.




              Coliforms
              Coliforms are defined as members of the family Enterobacteriaeceae which grow in the presence of bile salts and produce acid and gas from lactose within 48 hours at 37°C. In order to include anaerogenic bacteria and those which are nonlactose fermenters, it has been modified as the members of the Enterobacteriaeceae capable of growing galactosidase at 37°C that normally posses.The total coliform count is widely regarded as the most reliable indicator of potable water quality. However, the presence of coliforms not necessarily indicate faecal or sewage contamination, because, these organisms are present in large quantities in the environment.




              Faecal or thermotolerant coliforms
              These satisfy the criteria for coliforms but have the additional property of the ability to grow at a higher temperature 44°C.




              Faecal Escherichia coli
              These are defined as thermotolerant coliforms which ferment lactose (or) mannitol at 44°C with the production of acid and gas within 24 hours and also form indole from tryptophan at 44°C. The presence of E. coli is considered as the contamination of water with feces of human or animal origin.
              Faecal streptococci
              These are catalase negative, Gram positive cocci present in the intestinal tract of man and animals. These organisms have the Lancefield group D antigen, hydrolyse aesculin and can grow at 45°C, in the presence of azide and 40% bile. Such organisms which can survive 60°C for 30 min and can grow at 10°C at pH 9.6 and in 6.5% of sodium chloride (NaCl) belong to the genus Enterococcus (Enterococcus faecalis and E. faecium) .




              Clostridium perfringens
              The presence of this organism in water in the absence of other indicators of contamination of water implies remote or intermittent fecal pollution. Viruses in water are destroyed by chlorination. When the concentration of free residual chlorine is at least 0.5 mg per litre, for a minimum contact period of 30 minutes at pH below 8 and a turbidity of 1 nephelometric turbidity unit or less, protozoa such as Entamoeba histolytica, Giardia species and Balantidium coli may be present in the drinking water. Coliforms are not the reliable indicator of protozoal contamination.




              Collection of water samples
              Water is collected in heat sterilised bottles containing a sufficient volume of sodium thiosulphate to neutralise the bactericidal effect of any chlorine or chloramine in the water. For collection from tap, water is allowed to run to waste for 2–3 min. before collecting it into the bottle. When collecting water samples from lakes or streams the bottle is opened at a depth of about 30 cm with its mouth facing the current. At least 100 ml of water to be tested is collected in each bottle.
              After collecting the water in the bottle, the bottle is stoppered, and sent to the laboratory as quickly as possible within 6 hours keeping it in a cool container and protecting it from light.




              PRINCIPLE
              The following tests can be done for bacteriological analysis of water:
              1 Plate count.
              2 Detection of coliform bacteria and E. coli.
              a Presumptive coliform count: multiple tube technique.
              b Differential coliform test.
              c Membrane filtration method.
              3 Detection of faecal streptococci.
              4 Examination of Cl. perfringens, and
              5 Test for pathogenic bacteria.




              Plate count
              This consists of inoculating the nutrient agar with water to be tested and incubating the agar aerobically in parallel at 37°C for 1–2 days and at 22°C for 3 days. After incubation number of the colonies formed in the agar are counted. Those which grow at 37°C are associated with organic material of human or animal origin and those growing at a lower temperature are mainly saprophytes that normally inhabit water, soil, and vegetables. The agar count at 22°C gives an indication of the amount of decomposing organic matter in the water available for bacterial nutrition. Though these are non-pathogenic the greater the amount of organic matter present, the more likely is the water to be contaminated with parasitic and potentially pathogenic organisms.
              The agar count at 37°C is a more important index of dangerous pollution.
              Detection of coliform bacteria and E.coli
              Presumptive coliform test – Multiple tube
              technique
              The test is called presumptive, because of the presumption that the reactions are due to coliforms organisms. The count is made by adding varying quantities of water (0.1 ml–50 ml) to bile salt lactose peptone water with an indicator for acidity. Acid and gas formation indicate the growth of coliform bacilli.




              Differential coliform test
              This is called Eijkman test. This test is usually employed to find out whether the coliform bacilli detected in the presumptive test are E. coli or not. After the usual presumptive test, subcultures are made from all the bottles showing acid and gas to fresh tubes of single strength MacConkey medium already warmed to 37°C. They are incubated at 44°C for 24 hours. Those showing gas in Durham’s tubes contain E. coli. From the number of positive tubes obtained, results are read off the probability tables. Further confirmation of the presence of E. coli is done by testing for indole production and citrate utilization tests.




              Membrane filtration method
              A measured volume of water is filtered through a Millipore filter. All the bacteria present are retained on its surface. This is then placed on suitable media and incubated at the appropriate temperatures. Colonies on the surface of the membrane are counted. After 18 hours of incubation the presumptive coliform counts and detection of E. coli can be directly made.




              Detection of faecal streptococci
              Subcultures are made into tubes containing 5 ml of glucose azide broth from the positive bottles in the above test. Streptococcus faecalis if present produces acid in the medium within 18 hours at 45°C.




              Examination for Cl. perfringens
              Water is incubated in litmus milk medium at 37°C for 5 days, if positive, stormy fermentation occurs.




              Examination for pathognic bactrial cells test
              For other special pathogens like Salmonella, Vibrio, etc. corresponding special media are used.
              In this chapter Presumptive coliform test and differential coliform test will be discussed.




              REQUIREMENTS
              I -Equipments
              Bacteriological incubator, autoclave and water bath.




              II- Reagents
              MacConkey broth, brilliant green bile broth Preparation of MacConkey broth: This is prepared by mixing pancreatic digest of gelatin, 20 grams; lactose, 10 grams; bile salt, 5 grams; bromocresol purple, 0.01 grams and final pH (at 25°C) is adjusted at 7.3 ± 0.2.
              Preparation of double strength medium: It is prepared by suspending 35 grams in 500 ml of distilled water and heated to dissolve the medium completely. 50 ml and 10 ml of the media are dispensed into screw capped bottles with inverted Durham’s tubes and are sterilized by autoclaving at 15 lbs (121°C for 15 minutes).
              Preparation of single strength medium: It is prepared by suspending 3.5grams in 100 ml of distilled water. 5 ml quantities of the medium are dispensed in screw capped bottles with inverted Durham’s tubes and are sterilized by autoclaving at 15 lbs (121°C for 15 minutes).
              Preparation of brilliant green bile broth (BGBB): This is prepared by mixing peptic digest of animal tissue, 10 grams; lactose, 10 grams; ox gall, 20 grams and brilliant green, 0.0133 gm and adjusting the final pH (at 25°C) to 7.2 ± 0.2. 4 grams of the medium is suspended in 100 ml distilled water and mixed well. The media is distributed in 5ml volumes in test tubes with inverted Durham’s tubes and sterilized by autoclaving at 15 1bs pressure (121°C) for 15 minutes.




              III- Specimen
              Water specimen to be tested.




              PROCEDURE
              1- Collect 500 ml of water in a sterile bottle.
              2- Inoculate water sample immediately into the MacConkey broth medium.
              3- Inoculate 50 ml of water into 50 ml double strength media (1 bottle)
              4- Inoculate 10 ml of water into 10 ml double strength medium (5 bottles).
              5- Inoculate 1 ml of water into 5ml single strength medium (5 bottles).
              6- Incubate all the bottles at 37°C for 48 hours.
              7- Check for acid and gas after 24 hours and 48 hours.
              8 -Any positives are inoculated into brilliant green bile broth and peptone water.
              9 -Incubate at 44°C in a water bath overnight.




              QUALITY CONTROL
              Sterility of media and strength of media should be properly checked.




              OBSERVATIONS
              Observe for the presence of gas and production of indole. Presence of gas in brilliant green bile broth and indole production at 44°C is indicative of the presence of E. coli. For interpretation refer MacGrady’s table.




              RESULTS AND INTERPRETATION
              Presumptive coliform count The no. of bottles showing acid and gas is counted and compared with the MacGrady’s table. Result is expressed as- coliforms most probable no (MPN)/
              100ml. e.g. for Presumptive coliform count No. of tubes giving positive reaction 50 ml 10 ml 1 ml * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * * *1 * * * *2 * * * 2
              Result: Coliforms most probable no 10/100 ml.
              Differential coliform count
              The no of tubes showing positive results i.e. both gas productions in BGBB and Indole test at 44°C is compared with MacGrady’s table. Result is expressed a Escherichia coli Most probable No (MPN) / 100 ml. Eg. for Differential coliform counts: No. of tubes giving positive reaction.
              50 ml * 10 ml * *1 ml
              1 * * * * * 1 * * * * *1
              Results: Escherichia coli MPN—— 5 /100 ml
              Report: Unsatisfactory.
              Grades of the quality of drinking water supplied as determined by results of periodic Escherichia coli and coliform counts is listed in the table 84-1.






              *

              تعليق


              • #22
                جازاكم الله خيرا على كل ماتفضلتم به
                وجعله في ميزان حسناتكم

                تعليق


                • #23
                  أرجو من سعادتكم لو تكرمتم ذكر مصدر المعلومات القيمة هذه لأتمكن من كتابتها في التقرير النهائي
                  وجوزيتم خيرا على هذا

                  تعليق


                  • #24
                    السلام عليكم
                    الاخوه الاعضاء في منتدى المختبرات الطبيه
                    عندي سؤال في فحوصات المياة
                    وسؤالي هو اريد شرح عن طرق معالجه المياه من حيث (1)الغليان (2) الفلتره (3) الكلور
                    وكم تركيز الكلور المستخدم في معالجة المياه وكم يتم نضيف من الكلور للمياه
                    وشكرا لتعاونكم معنا

                    تعليق


                    • #25
                      السلام عليكم

                      أريد طريقة فحص بكتيريا Pseudomonas في الماء بطريقة ال filtration
                      الترشيح الغشائي بواسطه أجار asparag in broth base وكيفية تحضير الأجار
                      وكذلك طريقة فحص بكتيريا الكوليفورم وال ecoli بطريقة ال filtration

                      تعليق


                      • #26
                        الله يعطيك العافية استاذbo hadram على المعلومات القيمة
                        بس اذا كان عندك معلومات مفصلة عن طريقة الفحص الجرثومي بطريقة ماك-ريدي مع تحليل النتائج بكون شاكرة
                        الله يجزيك الخير

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