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Investigation of the Effect of Pasteurization on the Viability of Cryptosporidium Parvum in Cow's Milk by Propidium Monoazide Qpcr

dc.authorid Demir, Abdulbaki/0000-0002-6867-4410
dc.authorid Aydemir, Selahattin/0000-0002-0941-2779
dc.authorid Halidi, Ahmed Galip/0000-0002-1780-6671
dc.authorscopusid 57516565000
dc.authorscopusid 8261854400
dc.authorscopusid 57219095939
dc.authorscopusid 56741561500
dc.authorscopusid 57212309307
dc.authorscopusid 57210965593
dc.authorscopusid 57210965593
dc.authorwosid Aydemi̇r, Mehmet Emin/Abh-3062-2020
dc.authorwosid Aydemir, Selahattin/Acx-1253-2022
dc.authorwosid Arslan, Ali/W-3856-2018
dc.authorwosid Halidi, Ahemd Galip/Afl-9609-2022
dc.authorwosid Demir, Abdulbaki/Hns-5512-2023
dc.contributor.author Aydemir, Selahattin
dc.contributor.author Durmaz, Hisamettin
dc.contributor.author Aydemir, Mehmet Emin
dc.contributor.author Kilic Altun, Serap
dc.contributor.author Demir, Abdulbaki
dc.contributor.author Halidi, Ahmet Galip
dc.contributor.author Arslan, Ali
dc.date.accessioned 2025-05-10T17:18:41Z
dc.date.available 2025-05-10T17:18:41Z
dc.date.issued 2023
dc.department T.C. Van Yüzüncü Yıl Üniversitesi en_US
dc.department-temp [Aydemir, Selahattin] Van Yuzuncu Yil Univ, Fac Med, Dept Basic Med Sci, Dept Med Parasitol, Van, Turkiye; [Durmaz, Hisamettin; Aydemir, Mehmet Emin; Kilic Altun, Serap; Arslan, Ali] Harran Univ, Fac Vet Med, Dept Food Hyg & Technol, Sanliurfa, Turkiye; [Demir, Abdulbaki; Halidi, Ahmet Galip] Mus Alparslan Univ, Bulanik Vocat Sch, Mus, Turkiye en_US
dc.description Demir, Abdulbaki/0000-0002-6867-4410; Aydemir, Selahattin/0000-0002-0941-2779; Halidi, Ahmed Galip/0000-0002-1780-6671 en_US
dc.description.abstract Cow's milk, which is one of today's most important food sources, can be a reservoir for many patho-gens that create a risk to public health. One of these pathogens is Cryptosporidium parvum. The oocysts of C.parvum, an obligate intracellular parasite, cause infection when ingested orally. The oocysts scattered around with the feces of infected cows or calves can contaminate raw milk and this is frequently seen in dairy farms. The aim of this study was to investigate the viability of C.parvum by propidium monoazide (PMA)-quantitative polymerase chain reaction (qPCR) method after heat treatment applied to contami- nated raw cow's milk. For the study, 50 ml of unpasteurized cow's milk was contaminated with 5 X 105 C.parvum oocysts and portioned into 1.5 ml microcentrifuge tubes. Three groups, namely the control group, pasteurization group and boiling group were formed. No warming procedure was applied to the control group. In the pasteurization group, the milks in microcentrifuge tubes were poured into the wells of the dry block heater set to 71.7 degrees C and incubated for five seconds. At the end of the period, the milks were transferred to the wells of the cold metal tube, which was removed at-20 degrees C with the help of a micropipette, and incubated for five seconds. The milks in the boiling group were incubated for two minutes in a dry block heater set to 95 degrees C. After the heat treatment, the milks in microcentrifuge tubes were transferred to 10 ml centrifuge tubes, PBS was added to make the final volume 10 ml, and centrifuged at 4000 rpm for 20 minutes. After this process was repeated twice, 400 mu l of PBS was added to the precipitate remaining at the bottom, and the precipitate was homogenized. One sample of each group was applied with PMA, while PMA was not applied to the other sample. PMA-applied samples were incubated for five minutes at room temperature and in the dark, and then exposed to UV light for five minutes in the device with cooling feature. The oocysts were collected by centrifugation at 5000 g for five minutes. After DNA isolation from oocysts, SYBR Green real time PCR (Rt-PCR) was performed using primers amplifying the COWP gene region. As a result of SYBR Green Rt-PCR, the mean Ct values of the control without PMA, pasteurization and boiling groups were determined as 25 +/- 1.24, 23 +/- 0.98 and 26 +/- 1.03, respectively. While no peak was obtained in the boiling group after PMA application, the mean Ct values of the control and pasteurization groups were 28 +/- 1.38 and 31 +/- 1.46, respectively. As a result, it was concluded that live C.parvum cysts in milk could be detected by PMA-qPCR method and live oocysts could be found in pasteurized milk. en_US
dc.description.woscitationindex Science Citation Index Expanded
dc.identifier.doi 10.5578/mb.20239953
dc.identifier.endpage 666 en_US
dc.identifier.issn 0374-9096
dc.identifier.issue 4 en_US
dc.identifier.pmid 37885393
dc.identifier.pmid 37885393
dc.identifier.scopus 2-s2.0-85175278764
dc.identifier.scopusquality Q4
dc.identifier.startpage 660 en_US
dc.identifier.trdizinid 1206430
dc.identifier.uri https://doi.org/10.5578/mb.20239953
dc.identifier.uri https://hdl.handle.net/20.500.14720/9755
dc.identifier.volume 57 en_US
dc.identifier.wos WOS:001116646200007
dc.identifier.wosquality Q4
dc.language.iso en en_US
dc.publisher Ankara Microbiology Soc en_US
dc.relation.publicationcategory Makale - Uluslararası Hakemli Dergi - Kurum Öğretim Elemanı en_US
dc.rights info:eu-repo/semantics/openAccess en_US
dc.subject Pasteurization en_US
dc.subject Pma-Qpcr en_US
dc.subject Viability en_US
dc.subject Milk en_US
dc.title Investigation of the Effect of Pasteurization on the Viability of Cryptosporidium Parvum in Cow's Milk by Propidium Monoazide Qpcr en_US
dc.type Article en_US

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