Using species-specific repeat and PCR–RFLP in typing of DNA derived from blood of human and animal species

El‐Sayed, Yasser S.; Mohamed, Omnia Ismaeil; Ashry, Khaled M.; El-Rahman, Salah M. Abd

doi:10.1007/s12024-009-9117-5

Cited by 9 publications

(6 citation statements)

References 39 publications

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“…While immunological typing is generally sufficient when typing recipient and donor cats in practice, genotyping is preferred or performed in combination with immunological typing to assure the detection of the recessive alleles b and a c in type A and C cats when breeding cats [7]. Similarly, regular blood typing methods are complemented by genotyping assays to assure accuracy in blood typing in humans for several blood groups [32] [33]. Finally, crossmatching may be recommended prior to transfusing untyped and even A-B matched cats due to the potential presence of other naturally occurring alloantibodies and particularly for repeated transfusions > 4 days after the first transfusion [12][13] [34].…”

Section: Current Feline Typing Tools To Assure Blood Compatibilitymentioning

confidence: 99%

Neuigkeiten zur praktischen ABC-Blutgruppen-Bestimmung bei Katzen

Kehl

Truchet

Langbein-Detsch

et al. 2019

Tierarztl Prax Ausg K

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ZusammenfassungBis in die 1980er Jahre wurden die Blutgruppen bei Katzen als unwichtig angesehen. Seitdem gab es jedoch viele neue Erkenntnisse. Wir wissen heute: Das wichtigste Blutgruppensystem der Katze ist das AB-Blutgruppensystem (umbenannt als ABC-Blutgruppensystem) und umfasst die Blutgruppen A, B und AB (heute C genannt). Katzen haben natürlich vorkommende Antikörper gegen die Antigene der jeweils anderen Blutgruppe. Insbesondere Katzen mit Blutgruppe B haben hohe Titer an natürlich vorkommenden Anti-A-Alloantikörpern. Dadurch kann es bei A-B-inkompatiblen Bluttransfusionen und bei der sog. neonatalen Isoerythrolyse bei Welpen mit Typ A und C (AB) von Muttertieren mit Typ B zu Unverträglichkeitsreaktionen kommen. Um dies zu verhindern, ist es essenziell, für Zucht und im Vorfeld von Transfusionen die Blutgruppe und die zugrundeliegende Genetik zu kennen. Klinisch helfen serologische und genetische Tests. Diese Synopsis gibt einen aktuellen Überblick über die Blutgruppen, deren physiologische und genetische Grundlagen, mögliche Unverträglichkeitsreaktionen sowie die verschiedenen Nachweismethoden zu deren Vermeidung.

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Section: Current Feline Typing Tools To Assure Blood Compatibilitymentioning

confidence: 99%

Neuigkeiten zur praktischen ABC-Blutgruppen-Bestimmung bei Katzen

Kehl

Truchet

Langbein-Detsch

et al. 2019

Tierarztl Prax Ausg K

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“…In previous studies involving sequence analysis of 12S or 16S ribosomal RNA (rRNA) [2,3], methods using species-specific oligonucleotides (SSOs) [4] and classification by restriction fragment length polymorphisms (RFLPs) [5] were developed for identifying animal species in forensic settings. Currently, in wildlife forensic science, identification of animal species is commonly performed using cytochrome b (Cytb) or cytochrome c oxidase subunit I (COI) in mitochondrial DNA [6][7][8].…”

Section: Introductionmentioning

confidence: 99%

Non-specific peaks generated by animal DNA during human STR analysis: Peak characteristics and a novel analysis method for mixed human/animal samples

Inokuchi

Mizuno

Nakanishi

et al. 2018

Forensic Science International: Genetics

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“…Recently, molecular methods have been developed for DNA extracted from various sources and used for many purposes (e.g. economic, social, religious reasons, scientific, or industrial) (Bataille et al 1999;Kusama et al 2004;Girish et al 2005;El-Sayed et al 2010;Ali et al 2012).…”

Section: Introductionmentioning

confidence: 99%

Identifying the species of origin in commercial sausages in South Korea

Han

Cho

2016

Journal of Applied Animal Research

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This study aimed to develop a rapid and reliable method for identifying the species origin of the meat in commercial sausages using amplification patterns for mitochondrial DNA (mtDNA). Forty commercial sausages were purchased from retail markets and subjected to mtDNA analysis. Two mtDNA markers were used for amplifying the meat source DNA. To optimize the PCR conditions, gradient PCR reactions were carried out to determine the primer annealing temperatures, and real-time PCR was done to check the minimal amount of DNA solution and to examine the cross-reaction. PCR products were observed on the gels suggesting that DNA molecules may be useful in the identification of the meat source in processed sausages. A similarity search of the DNA sequences showed that they were from pig, chicken, and fish, as described on the product labels. The real-time PCR results showed that the PCR products were observed above 10 fg (0.01 pg)/μl concentrations in pig, chicken, and processed fish meat DNA. No significant amplification was found in cross-species. This PCR-based molecular method using mtDNA markers may provide useful information for food safety and traceability purposes by supplying molecular evidence for detecting and identifying the meat sources used in sausage production.

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Using species-specific repeat and PCR–RFLP in typing of DNA derived from blood of human and animal species

Cited by 9 publications

References 39 publications

Neuigkeiten zur praktischen ABC-Blutgruppen-Bestimmung bei Katzen

Neuigkeiten zur praktischen ABC-Blutgruppen-Bestimmung bei Katzen

Non-specific peaks generated by animal DNA during human STR analysis: Peak characteristics and a novel analysis method for mixed human/animal samples

Identifying the species of origin in commercial sausages in South Korea

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