Ginkgo biloba L., a “living fossil” and one of the most mysterious plant species, is the only extant representative of the isolated gymnosperm order Ginkgoales (Zhou, 2009). It became extinct in North America and Europe, and only survived the recurrent glaciation as a relic in China (Kwant, 2013). Recent molecular and ecological evidence strongly supports the existence of two refugia in China (Gong et al., 2008a, 2008b; Tang et al., 2012). Molecular data also confirmed an out-of-China distribution history mediated by anthropogenic introduction (Zhao et al., 2010). This fascinating plant has been cultivated worldwide for its medicinal and nutritional uses, its power as a source of artistic and religious inspiration, and its importance as one of the world's most popular street trees. Thus, it is imperative to increase our knowledge of its evolutionary history to support our efforts to conserve the refugial (natural) populations. Chloroplast DNA (cpDNA) sequences are prevalent markers used in population genetic studies. However, the relatively low resolution of cpDNA sequences of Ginkgo L. did not fully satisfy the inference of its evolutionary processes (Gong et al., 2008a, 2008b). Here, we report a set of polymorphic and monomorphic chloroplast microsatellite or simple sequence repeat (cpSSR) markers for G. biloba. They are expected to be particularly valuable, together with the published nuclear microsatellite markers (Yan et al., 2006, 2009), not only in inferring the evolutionary history but also for breeding of G. biloba.
METHODS AND RESULTS
Two complete chloroplast genomes of G. biloba (NC_016986 and AB684440) were downloaded from GenBank and manually aligned using Geneious version 4.8.5 (Drummond et al., 2008). Polymorphic mononucleotide repeats longer than nine nucleotides were spotted directly from the alignment. Di-, tri-, tetra-, and pentanucleotide motifs with a minimum of six repeats were identified from one of the chloroplast genomes using SSRHunter version 1.3 (Li and Wan, 2005). A total of 27 chloroplast simple sequence repeat loci (cpSSRs) were identified, including 22 mononucleotide repeats and five dinucleotide repeats. Primers for these 27 cpSSRs were designed using Primer Premier version 5.0 (Clarke and Gorley, 2001) following the criteria: (1) GC content 40–60%; (2) melting temperature (Tm) 50–60°C; (3) primer size 18–22 bp in length; and (4) amplicon size 100–400 bp in length.
Primer pairs were initially screened for amplification success using four individuals of G. biloba from a Tianmu Mountain population. Genomic DNA was extracted from silica gel–dried leaf materials using the cetyltrimethylammonium bromide (CTAB) method (Doyle and Doyle, 1987). PCR was performed in a 15-µL reaction mixture containing 60–90 ng genomic DNA, 0.75 U Taq polymerase (TaKaRa Biotechnology Co., Dalian, China), 0.8 µL 10× PCR buffer (MgCl2 free), 2 mM MgCl2, 0.12 mM dNTPs, and 0.33 µM of each primer, 6.67 mM bovine serum albumin (BSA, TaKaRa Biotechnology Co.). The amplification programs were as follows: initial denaturation at 94°C for 5 min; 30 cycles of 30 s at 94°C, 30 s at the optimized annealing temperature (Table 1), and extension for 40 s at 72°C; and a final extension step at 72°C for 10 min. Amplification products, along with a DL2000 DNA ladder (TaKaRa Biotechnology Co.), were electrophoresed on 2.0% agarose gels stained with ethidium bromide to assess successful amplification. Twenty-one of the 27 primer pairs produced amplicons matching the expected sizes. Polymorphisms of these 21 cpSSRs were assessed using 39 accessions from four populations, i.e., Jinfo Mountain, Chongqing Municipality (JF); Wuchuan, Guizhou Province (WC); Enshi, Hubei Province (ES); and Tianmu Mountain, Zhejiang Province (TM) (Appendix 1). As our previous studies (Gong et al., 2008a, 2008b) suggested, these populations are located in the two refugia. We repeated the experiments to verify the reproducibility of these amplicons. The forward primer of each pair was labeled with a fluorescent dye (6-FAM, HEX, or TAMRA). Amplification followed the conditions described above. Equal volumes of 10× diluted PCR products with three different dye-labeled primers were mixed with GeneScan 500 ROX Size Standard (Applied Biosystems, Carlsbad, California, USA). Fragment analyses were performed on a MegaBACE 1000 DNA Analysis System (GE Healthcare Biosciences, Pittsburgh, Pennsylvania, USA), and alleles were manually scored using GeneMarker version 1.97 (SoftGenetics, State College, Pennsylvania, USA). The resulting genotype data were analyzed using GenAlEx version 6.4.1 (Peakall and Smouse, 2006) to estimate number of alleles per locus (A) and unbiased haploid diversity (h).
TABLE 1.
Characteristics of 21 chloroplast microsatellite primers developed in Ginkgo biloba.
Eight out of the 21 stably amplified cpSSR markers were polymorphic in the four analyzed populations of G. biloba (Table 1). At the species level, the number of alleles per locus ranges from three to seven, and the unbiased haploid diversity per locus varies from 0.441 to 0.807 (Table 2). At the population level, the values of these two parameters range from one to five and from 0.250 to 0.810, respectively (Table 2). Population TM exhibits the highest level of genetic diversity (A = 3.9, h = 0.627), exceeding populations WC (2.1 and 0.384) and JF (2.0 and 0.295), while population ES shows the lowest values (1.8 and 0.277).
CONCLUSIONS
The first 21 chloroplast microsatellite markers were developed for G. biloba, including 13 monomorphic and eight polymorphic ones. The alleles of the eight polymorphic chloroplast loci were verified to be reliable. This set of novel polymorphic and monomorphic cpSSR markers provides a valuable tool for population genetic and phylogeographic investigations of G. biloba. They can also be useful for plant breeding companies, seed/sapling testing agencies, and the wider scientific community in identifying maternal parents and distinguishing cultivars of ginkgo. Furthermore, given the conservative nature of cpDNA loci, these markers might also be useful for other gymnospermous species, because three polymorphic cpDNA loci (i.e., trnK intron, trnS-trnG spacer [Gong et al., 2008a], and atpH-atpI spacer [Zhao et al., in preparation]) were successfully amplified in ginkgo using the universal markers.
TABLE 2.
Characteristics of eight polymorphic chloroplast microsatellite loci in four populations of Ginkgo biloba. a
LITERATURE CITED
Notes
[1] The authors thank Q. Y. Dai, Y. Sun, and L. Zheng for technical assistance with the experiment and suggestions on manuscript preparation. This research was supported by the National Natural Science Foundation of China (no. 31000102) and the Fundamental Research Funds for the Central Universities (no. 2012FZA6001).