Characterization of Fungus-Specific Microsatellite Markers in the Lichen-Forming Fungus Parmelina carporrhizans (Parmeliaceae)

David Alors; Francesco Dal Grande; Imke Schmitt; Ekaphan Kraichak; H. Thorsten Lumbsch; Ana Crespo; Pradeep K. Divakar

doi:10.3732/apps.1400081

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20 November 2014 Characterization of Fungus-Specific Microsatellite Markers in the Lichen-Forming Fungus Parmelina carporrhizans (Parmeliaceae)

David Alors, Francesco Dal Grande, Imke Schmitt, Ekaphan Kraichak, H. Thorsten Lumbsch, Ana Crespo, Pradeep K. Divakar

Author Affiliations +

Applications in Plant Sciences, 2(12): (2014). https://doi.org/10.3732/apps.1400081

Parmelina carporrhizans (Taylor) Poelt & Vêzda (Parmeliaceae) is a sexually reproducing foliose lichen species that has long been considered synonymous with the morphologically similar P. quercina (Willd.) Hale. Thus, the geographic distribution and degree of conservation of both species are poorly known (Argüello et al., 2007; Clerc and Truong, 2008). These two species are largely allopatric but they occasionally overlap, being apparently parapatric depending on the climatic conditions. Hence they possibly may be used as indicators of climate change. Parmelina carporrhizans has an Atlantic-Mediterranean distribution in Europe. It is abundant in the central-western Iberian Peninsula in the humid supra- and mesomediterranean level on deciduous Quercus L. vegetation (Argüello et al., 2007; Nuñez-Zapata, 2013). The species also occurs across open forest and in isolated trees above the Canarian monteverde forest in central Macaronesia from 800 to 1500 m and is locally common on Gran Canaria. Further, P. carporrhizans is listed as “vulnerable” on the Red Lists of England and Wales (Church et al., 1996; Woods, 2010). Despite these conservation concerns, our knowledge of the population genetics of this species is currently limited.

We developed 11 microsatellite markers for high-resolution population studies in P. carporrhizans to provide a better understanding of its genetic diversity, gene flow, and population structure. The enhanced knowledge will allow us to implement an informed conservation plan and investigate potential impacts of climate change on this narrowly distributed species. In addition, we also investigate whether this set of high-resolution microsatellite markers can be applied to other closely related species in the genus Parmelina Hale.

METHODS AND RESULTS

We isolated the mycobiont of P. carporrhizans from ascospores of two thalli (deposited in the herbarium of the Universidad Complutense de Madrid [MAF], Madrid, Spain: MAF-Lich 19191 and MAF-Lich 19192) collected in Cuevas del Valle, Spain (40°18′28.4″N, 5°00′39.0″W), in October 2012, following the inverted Petri dish method (Ahmadjian, 1993). We germinated spores in Basal Bold Medium (Deason and Bold, 1960), and after two weeks these were transferred to corn meal agar (CMA) and malt yeast (Honegger et al., 2004), where the cultures were grown for four months.

Prior to DNA extraction, we removed secondary metabolites with acetone, and then crushed the samples with pestles in liquid nitrogen and extracted genomic DNA with the DNeasy Plant Kit (QIAGEN, Redwood City, California, USA) according to the manufacturer's instructions.

To confirm the identity of the mycobiont cultures, we amplified the internal transcribed spacer (ITS) region of the nuclear rDNA from the axenic cultured tissues. Genomic DNA (10–25 ng) was used for PCR amplifications. Primers, PCR, and cycle sequencing conditions were the same as described previously (Argüello et al., 2007). Sequencing was conducted on an ABI 3730 DNA analyzer (Applied Biosystems, Foster City, California, USA) at Centro de Genómica y Proteómica del Parque Científico de Madrid. The identity of the sequences and specimens were confirmed using the MegaBLAST search function in GenBank. ITS sequences were deposited in GenBank (accession numbers KM357892 and KM357893).

Table 1.

Overview of the microsatellite loci and associated primer sets successfully developed for Parmelina carporrhizans and deposited in the National Center for Biotechnology Information (NCBI) database.

From the extracted DNA, approximately 0.5 µg of genomic DNA was used to construct an Illumina library using the Nextera XT multiplex paired-end kit (Illumina, San Diego, California, USA). The library was paired-end sequenced using an Illumina HiSeq 2000 with 100 cycles (version 3 chemistry). Standard Illumina protocols ( http://www.illumina.com/) were used to generate the library. Sequencing was carried out at the Stab Vida Laboratory (Madan Parque, Caparica, Portugal). Illumina reads were assembled to contigs using the “De novo assembly” option of the CLC Genomics Workbench version 6.0.4 (CLC bio, Aarhus, Denmark). A total of 38,115,484 reads with an average length of 69.06 bases and a total of 2,632,336,717 bases were recovered. De novo assembly produced 31,035 contigs (N50 = 3615 bp) with an average of approximately 73× coverage, which totaled 36.2 Mbp of genome data.

All the contigs were screened for microsatellites using MSATCOMMANDER 1.0.8 (Faircloth, 2008), accepting di-, tri-, tetra-, penta-, and hexanucleotide repeats of ≥15. We found 63 contigs containing microsatellite sequences with 15 to 20 repeats (29 dinucleotides, 24 trinucleotides, 7 tetranucleotides, 2 pentanucleotides, and 1 hexanucleotide). From these contigs, we designed short primers of 19–21 bp in length with the program Primer3 using default parameters (Rozen and Skaletsky, 2000), expecting some transferability within the genus as reported in other lichen mycobionts (Jones et al., 2012; Devkota et al., 2014). We excluded contigs with short flanking regions, as well as repeated motifs on the flanking region, and selected primer pairs with amplicons between 100 and 400 bp. Finally, an M13 tag (5′-TGTAAAACGACGGCCAGT-3′) was appended to forward primers for subsequent amplification.

Microsatellite PCRs were performed in a 10-µL reaction volume containing ∼0.5–5 ng of genomic DNA, 1× Type-it Multiplex Master Mix (QIAGEN, Hilden, Germany), 0.15 µM of reverse primer, 0.01 µM of M13-tailed forward primer, and 0.15 µM of dyer-M13-labeled primer (Schuelke, 2000). PCRs were carried out with an initial 5-min denaturation at 94°C; followed by 35 cycles of 94°C for 30 s, 57°C for 45 s, and 72°C for 45 s; and a final extension of 72°C for 30 min.

We tested the 24 primer pairs with seven accessions of P. carporrhizans from different areas of its distribution range and one accession of P. tiliacea (Hoffm.) Hale (MAF-Lich 17252); see Appendix 1 for specific localities. Out of these 24 primers, only 12 pairs successfully amplified all of the P. carporrhizans samples, and four pairs amplified in P. tiliacea. We then tested this subset of 12 primer pairs for variability with 30 samples of P. carporrhizans from Gran Canaria and Tenerife (MAF-Lich numbers 19123–19152; Appendix 1), as well as one accession each of P. tiliacea and P. cryptotiliacea Crespo & Núñez-Zapata (MAF-Lich 19403 and MAF-Lich 19402, respectively). Eight of these primer pairs (Pcar1-Pcar8) amplified all P. carporrhizans samples, while the other three (Pcar9-Pcar11) had 3.3–10% missing data. Four of these primer pairs (Pcar3, Pcar5, Pcar7, Pcar9) amplified in P. tiliacea and none amplified in P. cryptotiliacea. We deposited these 11 primer sequences in GenBank (Table 1); other primer pairs were excluded due to their low amplification rate (<60%). Our limited cross-species amplification results suggest that it may be possible to use some of these markers in other species of the P. carporrhizans clade (Nuñez-Zapata, 2013).

Polymorphism within the eight microsatellite loci that amplified across all P. carporrhizans samples was determined by counting the number of alleles and calculating Nei's unbiased haploid diversity (Table 2) using GenAlEx version 6.41 (Peakall and Smouse, 2006). The number of alleles ranged from four to 14, and the average unbiased diversity was 0.76, a relatively high number for just 30 individuals from a small geographic area. No identical multilocus genotypes were found among the samples as is expected for a sexually reproducing lichen-forming fungus.

Table 2.

Number of alleles (A) and Nei's unbiased genetic diversity (H_e) of the eight polymorphic microsatellite loci that were amplified with 100% success across 30 samples from the Canary Islands.

CONCLUSIONS

We developed 11 polymorphic fungus-specific microsatellite markers to facilitate studies of population genetics in P. carporrhizans. Eight of the 11 microsatellite primer pairs are being used to analyze P. carporrhizans populations. The results from future population genetic studies will help inform us on population responses to global changes, clarify the mechanisms of speciation, as well as define populations of this narrowly distributed species for conservation purposes.

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Appendices

Appendix 1.

Voucher information for specimens of Parmelina carporrhizans, P. cryptotiliacea, and P. tiliacea used in this study. All the specimens are deposited in the Lichen section of MAF herbarium, Faculty of Pharmacy, Universidad Complutense de Madrid, Madrid, Spain (MAF-Lich).^a

Appendix 1. (cont)

Voucher information for specimens of Parmelina carporrhizans, P. cryptotiliacea, and P. tiliacea used in this study. All the specimens are deposited in the Lichen section of MAF herbarium, Faculty of Pharmacy, Universidad Complutense de Madrid, Madrid, Spain (MAF-Lich).^a

Appendix 1. (cont)

Voucher information for specimens of Parmelina carporrhizans, P. cryptotiliacea, and P. tiliacea used in this study. All the specimens are deposited in the Lichen section of MAF herbarium, Faculty of Pharmacy, Universidad Complutense de Madrid, Madrid, Spain (MAF-Lich).^a

Notes

[1] The authors acknowledge funding from the Ministerio de Ciencia e Innovación de España (projects CGL2010-21646/BOS, CGL2011-25003, and CGL2013-42498-P).

Citation Download Citation

David Alors, Francesco Dal Grande, Imke Schmitt, Ekaphan Kraichak, H. Thorsten Lumbsch, Ana Crespo, and Pradeep K. Divakar "Characterization of Fungus-Specific Microsatellite Markers in the Lichen-Forming Fungus Parmelina carporrhizans (Parmeliaceae)," Applications in Plant Sciences 2(12), (20 November 2014). https://doi.org/10.3732/apps.1400081

Received: 21 August 2014; Accepted: 17 October 2014; Published: 20 November 2014

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