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      Phylogeography and ecological niche modelling inEugenia uniflora(Myrtaceae) suggest distinct vegetational responses to climate change between the southern and the northern Atlantic Forest

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          The Community Climate System Model Version 3 (CCSM3)

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            Use of DNA barcodes to identify flowering plants.

            Methods for identifying species by using short orthologous DNA sequences, known as "DNA barcodes," have been proposed and initiated to facilitate biodiversity studies, identify juveniles, associate sexes, and enhance forensic analyses. The cytochrome c oxidase 1 sequence, which has been found to be widely applicable in animal barcoding, is not appropriate for most species of plants because of a much slower rate of cytochrome c oxidase 1 gene evolution in higher plants than in animals. We therefore propose the nuclear internal transcribed spacer region and the plastid trnH-psbA intergenic spacer as potentially usable DNA regions for applying barcoding to flowering plants. The internal transcribed spacer is the most commonly sequenced locus used in plant phylogenetic investigations at the species level and shows high levels of interspecific divergence. The trnH-psbA spacer, although short ( approximately 450-bp), is the most variable plastid region in angiosperms and is easily amplified across a broad range of land plants. Comparison of the total plastid genomes of tobacco and deadly nightshade enhanced with trials on widely divergent angiosperm taxa, including closely related species in seven plant families and a group of species sampled from a local flora encompassing 50 plant families (for a total of 99 species, 80 genera, and 53 families), suggest that the sequences in this pair of loci have the potential to discriminate among the largest number of plant species for barcoding purposes.
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              A Two-Locus Global DNA Barcode for Land Plants: The Coding rbcL Gene Complements the Non-Coding trnH-psbA Spacer Region

              Background A useful DNA barcode requires sufficient sequence variation to distinguish between species and ease of application across a broad range of taxa. Discovery of a DNA barcode for land plants has been limited by intrinsically lower rates of sequence evolution in plant genomes than that observed in animals. This low rate has complicated the trade-off in finding a locus that is universal and readily sequenced and has sufficiently high sequence divergence at the species-level. Methodology/Principal Findings Here, a global plant DNA barcode system is evaluated by comparing universal application and degree of sequence divergence for nine putative barcode loci, including coding and non-coding regions, singly and in pairs across a phylogenetically diverse set of 48 genera (two species per genus). No single locus could discriminate among species in a pair in more than 79% of genera, whereas discrimination increased to nearly 88% when the non-coding trnH-psbA spacer was paired with one of three coding loci, including rbcL. In silico trials were conducted in which DNA sequences from GenBank were used to further evaluate the discriminatory power of a subset of these loci. These trials supported the earlier observation that trnH-psbA coupled with rbcL can correctly identify and discriminate among related species. Conclusions/Significance A combination of the non-coding trnH-psbA spacer region and a portion of the coding rbcL gene is recommended as a two-locus global land plant barcode that provides the necessary universality and species discrimination.
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                Author and article information

                Journal
                Botanical Journal of the Linnean Society
                Bot. J. Linn. Soc.
                Wiley
                00244074
                November 2016
                November 2016
                October 05 2016
                : 182
                : 3
                : 670-688
                Affiliations
                [1 ]Programa de Pós-Graduação em Genética e Biologia Molecular; Universidade Federal do Rio Grande do Sul (UFRGS); Av. Bento Goncalves 9500 91501970 Porto Alegre Rio Grande do Sul Brazil
                [2 ]Departamento de Botânica; Universidade Federal do Estado do Rio de Janeiro (UNIRIO); Av. Pasteur 458 22290-255 Rio de Janeiro Brazil
                [3 ]Centro de Biotecnologia e Departamento de Biofísica; UFRGS; Av Bento Goncalves 9500, Predio 43431 sala 213 91501-970 Porto Alegre Rio Grande do Sul Brazil
                Article
                10.1111/boj.12473
                c9e42b03-3b5c-4c96-85e2-94aa8cc340d7
                © 2016

                http://doi.wiley.com/10.1002/tdm_license_1

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