Gene/Protein Disease Symptom Drug Enzyme Compound
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Query: EC:3.2.1.26 (invertase)
 4,927 document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)

The occurrence of intermixing, especially that resulting from genetically modified (GM) species, is increasingly becoming a problem in the delicate chain of feed and food quality control. Thus, a strategy is needed for precisely quantifying the presence of intermixing. An analytical assay based on real-time PCR has been developed; it can ascertain the extent of unexpected intermixing of GM soybean with maize meal. Three soybean-maize mix levels, with soybean intermix percentages of, respectively, 0.1, 0.5, and 1%, were prepared to simulate samples containing traces of soybean. As calibrator standards, ad hoc multiple-target pGEM-T plasmids containing soybean and maize reference genes in a 1:1 ratio were constructed. Four different maize endogenous genes, alcohol dehydrogenase 1 (adh1), high-mobility group protein a (hmga), invertase 1 (ivr1), and zein (zein), were assessed, each combined with the soybean endogenous lectin 1 (lect1) gene. Plasmids containing adh1-lect1 and zein-lect1 genes were found to be the most reliable calibration systems for this analysis, providing precise and accurate quantification results. Measuring the percentage of GM soybean intermixing makes it possible to calculate the actual transgenic component of the total sample.
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PMID:Development of a real-time PCR method based on duplo target plasmids for determining an unexpected genetically modified soybean intermix with feed components. 1730 Jan 50

A reliable PCR reference assay for relative genetically modified organism (GMO) quantification must be specific for the target taxon and amplify uniformly along the commercialised varieties within the considered taxon. Different reference assays for maize (Zea mays L.) are used in official methods for GMO quantification. In this study, we evaluated the reliability of eight existing maize reference assays, four of which are used in combination with an event-specific polymerase chain reaction (PCR) assay validated and published by the Community Reference Laboratory (CRL). We analysed the nucleotide sequence variation in the target genomic regions in a broad range of transgenic and conventional varieties and lines: MON 810 varieties cultivated in Spain and conventional varieties from various geographical origins and breeding history. In addition, the reliability of the assays was evaluated based on their PCR amplification performance. A single base pair substitution, corresponding to a single nucleotide polymorphism (SNP) reported in an earlier study, was observed in the forward primer of one of the studied alcohol dehydrogenase 1 (Adh1) (70) assays in a large number of varieties. The SNP presence is consistent with a poor PCR performance observed for this assay along the tested varieties. The obtained data show that the Adh1 (70) assay used in the official CRL NK603 assay is unreliable. Based on our results from both the nucleotide stability study and the PCR performance test, we can conclude that the Adh1 (136) reference assay (T25 and Bt11 assays) as well as the tested high mobility group protein gene assay, which also form parts of CRL methods for quantification, are highly reliable. Despite the observed uniformity in the nucleotide sequence of the invertase gene assay, the PCR performance test reveals that this target sequence might occur in more than one copy. Finally, although currently not forming a part of official quantification methods, zein and SSIIb assays are found to be highly reliable in terms of nucleotide stability and PCR performance and are proposed as good alternative targets for a reference assay for maize.
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PMID:Evaluation of the reliability of maize reference assays for GMO quantification. 2006 84