Microsatellites are codominantly inherited nuclear-DNA markers (Wright and Bentzen, 1994) that are now commonly used to assess both stock structure and the effective population size of exploited fishes (Turner et al., 2002; Chistiakov et al., 2006; Saillant and Gold, 2006). Multiplexing is the combination of polymerase chain reaction (PCR) amplification products from multiple loci into a single lane of an electrophoretic gel (Olsen et al., 1996; Neff et al., 2000) and is accomplished either by coamplification of multiple loci in a single reaction (Chamberlain et al., 1988) or by combination of products from multiple single-locus PCR amplifications (Olsen et al., 1996). The advantage of multiplexing micro-satellites lies in the significant reduction in both personnel time (labor) and consumable supplies generally required for large genotyping projects (Neff et al., 2000; Renshaw et al., 2006)

Berry, Philip

Gold, John R.

Lem, Siya

Renshaw, Mark A.

Saillant, Eric

Aquatic Commons

ART & E UATIONS ARE LINKED
436 
Q 
Microsatellite multiplex panels for genetic studies 
of gray snapper (Lutjanus griseus) and 
lane snapper (Lutjanus synagris) 
Mark A. Renshaw 
Eric Saillant 
Siya Lem 
Philip Berry 
John R. Gold 
Email address for M. A. Renshaw: mrenshaw@ag.tamu.edu 
Center for Biosystematics and Biodiversity 
Texas A&M University, TAMU−2258 
College Station, Texas 77843−2258 
Microsatellites are codominantly 
inherited nuclear-DNA markers 
(Wright and Bentzen, 1994) that are 
now commonly used to assess both 
stock structure and the effective 
population size of exploited fishes 
(Turner et al., 2002; Chistiakov et 
al., 2006; Saillant and Gold, 2006). 
Multiplexing is the combination of 
polymerase chain reaction (PCR) 
ampliﬁcation products from multiple 
loci into a single lane of an electropho-
retic gel (Olsen et al., 1996; Neff et 
al., 2000) and is accomplished either 
by co-amplification of multiple loci 
in a single reaction (Chamberlain et 
al., 1988) or by combination of prod-
ucts from multiple single-locus PCR 
amplifications (Olsen et al., 1996). 
The advantage of multiplexing micro-
satellites lies in the signiﬁcant reduc-
tion in both personnel time (labor) 
and consumable supplies generally 
required for large genotyping proj-
ects (Neff et al., 2000; Renshaw et 
al., 2006). 
In this note, we report the devel-
opment of multiplex panels of mic-
rosatellites that will facilitate popu-
lation-level genetic studies of both 
gray (Lutjanus griseus) and lane 
(L. synagris) snappers. The overex-
ploitation of Gulf red snapper (L. 
campechanus) in U.S. waters and the 
increasing restrictions on both com-
mercial and recreational red snap-
per catches (Gillig et al., 2001) have 
led to increased ﬁshing pressure on 
other snapper species (Fischer et al., 
2005), including both gray (Burton, 
2001; Fischer et al., 2005) and lane 
snappers (GMFMC1). Although nei-
ther species has yet been classiﬁed 
as “overﬁshed” or subject to “overﬁsh-
ing,” the increased exploitation of the 
two species could jeopardize these 
snapper resources in the future. In 
this study, we optimized multiplex 
panels for gray and lane snappers 
from among microsatellite markers 
designed originally for red snapper 
by Gold et al. (2001) and vermillion 
snapper (Rhomboplites aurorubens) 
by Bagley and Geller (1998). 
Materials and methods 
Samples of gray and lane snappers 
were obtained off the west coast of 
Florida during April of 2004. Fin clips 
and pieces of liver were preserved in 
95% ethanol, brought to the labora-
tory, and stored at room temperature. 
Genomic DNA was extracted by using 
an alkaline-lysis method (Saillant et 
al., 2002) and stored at −20°C. 
1 GMFMC (Gulf of Mexico Fishery 
Management Council). 2005. Final 
amendment to the FMPs for: reef fish 
(Amendment 25) and coastal migratory 
pelagics (Amendment 17) for extending 
the charter vessel/headboat permit mor-
atorium (including SEIS/RIR/IRFA), 
111 p. Gulf of Mexico Fishery Man-
agement Council, 3018 North U.S. 
Highway 301, Suite 1000, Tampa, FL 
33619−2272. 
Microsatellites were ﬁrst evaluated 
in single-locus (simplex) reactions in 
order to determine the size range 
and ease of scoring of PCR products 
in each species. PCR ampliﬁcations 
were performed in 11.5-μL volumes 
comprising 1.5 μL of DNA (approxi-
mately 50 ng), 1 μL of 10× reaction 
buffer [50 mm KCl, 10 mm Tris, 1% 
Triton-X 100], 0.75 U Taq DNA poly-
merase (Invitrogen, Carlsbad, CA), 
200 μm of each dNTP, 1 mm MgCl2, 
and various quantities of PCR prim-
ers. One PCR primer of each pair 
was labeled with one of three ﬂuores-
cent dyes from set D (Applied Biosys-
tems, Foster City, CA): FAM, HEX, or 
NED. Fragment analysis was carried 
out on an ABI PRISM 377 automated 
DNA sequencer (Applied Biosystems, 
Foster City, CA). Allele size was 
estimated by using the GENESCAN-
400HD [ROX] size standard (Applied 
Biosystems, Foster City, CA); allele 
size estimation was performed with 
GENESCAN 3.1.2 (Applied Biosystems, 
Foster City, CA) and allele calling 
was performed in GENOTYPER, version 
2.5 (Applied Biosystems, Foster City, 
CA). Multiplex tests were performed 
only on those microsatellites that am-
pliﬁed successfully and yielded PCR 
products that were easy to score; loci 
not meeting these criteria were elim-
inated from subsequent analyses. 
Initial multiplex PCR amplifica-
tions were performed by using the 
three multiplex panels designed to 
amplify 20 microsatellite loci in red 
snapper (Renshaw et al., 2006). At 
ﬁrst, PCR primer concentrations fol-
lowed those outlined in Renshaw et 
al. (2006), and changes were made 
according to the relative success of 
ampliﬁcations at each microsatellite 
within a particular multiplex. Mic-
rosatellites that failed to amplify in 
multiplex reactions were optimized 
in simplex reactions. Additional PCR 
Manuscript submitted 14 September 2006 
to the Scientiﬁc Editor’s Ofﬁce. 
Manuscript approved for publication 
9 November 2006 by the Scientiﬁc Editor. 
Fish. Bull. 105:436-439 (2007). 
PREFLIGHT GOOD TO GO
437 NOTE Renshaw et al.: Microsatellite multiplex panels for genetic studies of Lutjanus griseus and Lutjanus synagris 
Table 1 
Technical details on ampliﬁcation of microsatellite loci in gray snapper (Lutjanus griseus) and lane snapper (L. synagris). 
Included in the table are the multiplex polymerase chain reaction (PCR) panel, primer quantities, and ﬂuorescent dye labels 
(Set D; Applied Biosystems, Foster City, CA). PCR protocols, including appropriate annealing temperatures, correspond to those 
outlined in Renshaw et al. (2006). Primer sequences for Lca and Prs microsatellites are given in Gold et al. (2001); those for Ra 
microsatellites are given in Bagley and Geller (1998). 
Species Panel Microsatellite Quantity (pmol) ABI dye PCR protocol 
Lutjanus griseus 1 Lca 20 5 FAM Touchdown II 
Lca 43 4 FAM 56o 
Prs 260 1.5 FAM 53o 
Ra 1 3.5 HEX 50o 
2 Prs 137 7 FAM Touchdown II 
Prs 275 6 FAM 54o 
Prs 328 0.8 FAM 52o 
Ra 6 2 NED 50o 
3 Lca 22 2.5 FAM Touchdown I 
Lca 91 8 FAM 56o−50.5o 
Lca 107 6.5 HEX 50o 
simplex Prs 221 5 HEX Same as panel 2 
simplex Prs 240 5 HEX Same as panel 3 
simplex Ra 7 5 NED Same as panel 3 
Lutjanus synagris 1 Lca 20 5 FAM Touchdown II 
Prs 248 5 NED 52o 
Prs 260 1.5 FAM 50o 
Prs 303 1.5 NED 48o 
Ra 1 7.5 NED 
Ra 4 5 HEX 
2 Prs 275 4 FAM Touchdown II 
Prs 328 1 FAM 52o 
Ra 2 3.5 FAM 50o 
Ra 6 3 NED 48o 
3 Lca 22 1 FAM Touchdown II 
Lca 91 8 FAM 52o 
Prs 240 9 HEX 50o 
Prs 333 3 HEX 48o 
Ra 7 5 NED 
primers (Ra 1, Ra 2, and Ra 4) designed by Bagley and 
Geller (1998) for vermillion snapper microsatellites were 
tested in simplex reactions as described above and la-
beled with one ﬂuorescent dye to allow integration into 
one of the three multiplex panels. 
Multiplex PCR ampliﬁcations initially followed the 
Touchdown I and II protocols outlined in Renshaw et al. 
(2006). Touchdown PCR protocols enable the ampliﬁca-
tion of multiple loci with different optimal annealing 
temperatures. The former (Touchdown I) protocol in-
volved a one-half degree drop in annealing temperature 
with each subsequent cycle, for a total of 12 cycles, fol-
lowed by 30 cycles at a bottom annealing temperature 
that was 6°C below the initial annealing temperature; 
the latter (Touchdown II) protocol featured a three-step 
drop in annealing temperature with seven cycles at an 
initial annealing temperature, followed by seven cycles 
at a lower annealing temperature, followed by 28 cycles 
at a bottom annealing temperature that was 4−6°C 
below the initial annealing temperature. Changes were 
made to optimize multiplex panels individually for each 
species. These changes included 1) removal of various 
primers and addition of others, and 2) modiﬁcation of 
annealing temperatures and species-speciﬁc differences 
in primer concentrations. 
Once multiplex or simplex protocols were developed for 
the two species, DNA from 28 individuals of each spe-
cies was assayed across all optimized loci. Genetic vari-
ability of microsatellites in each species was measured 
by the number of alleles, expected heterozygosity (gene 
diversity), and observed heterozygosity. Fisher’s exact 
test was used to evaluate loci for signiﬁcant departures 
from Hardy-Weinberg equilibrium expectations. Three 
common causes for genotyping errors—null alleles, 
large allele dropout, and stuttering—were assessed with 
MICRO-CHECKER (Van Oosterhout et al., 2004). 
438 Fishery Bulletin 105(3) 
Table 2 
Summary data for microsatellites ampliﬁed from 28 gray snapper (Lutjanus griseus) and 28 lane snapper (L. synagris). Data for 
each microsatellite include number of alleles (NA), size range (in base pairs) of detected alleles, expected (HE) and observed (HO) 
heterozygosity, and probability (PHW) of conformity to Hardy-Weinberg equilibrium expectations. Lca and Prs microsatellites 
were developed initially for red snapper (L. campechanus) (Gold et al., 2001), and Ra microsatellites were developed initially for 
vermillion snapper (Rhombloplites aurorubens) (Bagley and Geller, 1998). 
Species Microsatellite NA Size range HE/HO PHW 
Lutjanus griseus Lca 20 4 216−222 0.707/0.643 0.721 
Lca 22 5 242−252 0.593/0.500 0.050 
Lca 43 2 176−188 0.195/0.214 1.000 
Lca 91 2 134−136 0.036/0.036 1.000 
Lca 107 6 112−144 0.771/0.750 0.266 
Prs 137 7 127−141 0.794/0.679 0.075 
Prs 221 4 235−245 0.566/0.714 0.448 
Prs 240 4 210−220 0.642/0.679 0.963 
Prs 260 9 105−129 0.847/1.000 0.060 
Prs 275 5 156−168 0.548/0.571 0.343 
Prs 328 3 202−206 0.527/0.464 0.842 
Ra 1 7 149−171 0.594/0.571 0.081 
Ra 6 15 113−155 0.926/0.679 0.000 
Ra 7 3 154−158 0.200/0.143 0.127 
Lutjanus synagris Lca 20 12 234−262 0.810/0.571 0.009 
Lca 22 8 234−256 0.712/0.679 0.257 
Lca 91 7 139−153 0.601/0.679 0.263 
Prs 240 5 192−202 0.592/0.538 0.484 
Prs 248 17 224−260 0.938/0.893 0.402 
Prs 260 4 92−120 0.292/0.321 1.000 
Prs 275 2 154−156 0.036/0.036 1.000 
Prs 303 4 135−141 0.690/0.643 0.724 
Prs 328 5 198−214 0.631/0.571 0.499 
Prs 333 12 152−180 0.870/0.821 0.327 
Ra 1 9 141−163 0.806/0.893 0.587 
Ra 2 6 82−100 0.704/0.821 0.972 
Ra 4 9 59−99 0.787/0.821 0.660 
Ra 6 4 118−124 0.384/0.464 0.770 
Ra 7 4 177−187 0.612/0.536 0.578 
Results and discussion 
A total of 14 microsatellites (11 in three multiplex panels 
and 3 in simplex reactions) were optimized for gray snap-
pers, and 15 microsatellites (in three multiplex panels) 
were optimized for lane snappers. The multiplex and 
simplex formats are presented in Table 1 and include for 
each microsatellite the ﬂuorescent label (Applied Biosys-
tems, Foster City, CA), primer quantity, PCR protocol, 
and optimized annealing temperatures. Genotype sum-
mary data from 28 individuals (in both species) are given 
in Table 2; data for each microsatellite include number 
of alleles, size range of alleles detected, expected and 
observed heterozygosity, and probability of conformity 
to Hardy-Weinberg equilibrium expectations. 
For gray snappers, the number of alleles per microsat-
ellite ranged from two (Lca 43 and Lca 91) to 15 (Ra 6), 
and expected and observed heterozygosity per microsat-
ellite ranged from 0.036 (Lca 91) to 0.926 (Ra 6) and 
from 0.036 (Lca 91) to 1.000 (Prs 260), respectively. 
Only one microsatellite (Ra 6) deviated signiﬁcantly 
(P<0.05) from Hardy-Weinberg equilibrium expecta-
tions after sequential Bonferroni correction (Rice, 
1989). Analysis with MICRO-CHECKER (Van Oosterhout 
et al., 2004) indicated the possible occurrence of null 
alleles at Ra 6. 
For lane snappers, the number of alleles per micro-
satellite ranged from two (Prs 275) to 17 (Prs 248), and 
expected and observed heterozygosity per microsatellite 
ranged from 0.036 (Prs 275) to 0.938 (Prs 248) and from 
0.036 (Prs 275) to 0.893 (Prs 248 and Ra 1), respective-
ly. None of the 15 microsatellites deviated signiﬁcantly 
from Hardy-Weinberg equilibrium expectations after 
sequential Bonferroni correction (Rice, 1989). Analysis 
with MICRO-CHECKER indicated the possibility of null al-
leles at one microsatellite (Lca 20) where the probability 
439 NOTE Renshaw et al.: Microsatellite multiplex panels for genetic studies of Lutjanus griseus and Lutjanus synagris 
of deviation from Hardy-Weinberg equilibrium expecta-
tions was signiﬁcant (P=0.009) before Bonferroni cor-
rection. One locus, Lca 91, exhibited a one base-pair 
shift (rather than the two base-pair shifts expected 
from dinucleotide repeats) in samples of lane snapper; 
this difference in shift could generate scoring problems 
in future genotyping efforts. 
The costs of large genotyping projects can be substan-
tially reduced through the combination of multiple loci 
in single PCR ampliﬁcations (Renshaw et al., 2006). 
The reduction in costs could enable researchers to in-
crease sample sizes, possibly allowing for the inclusion 
of additional year classes for temporal studies or could 
extend a proposed sampling range to include more of 
the geographic distribution of a species. The multiplex 
panels and simplex reactions developed in the present 
study will provide critical tools for future population-
level genetic studies designed to identify ﬁshery man-
agement units and to monitor changes in genetic effec-
tive population size for both gray and lane snappers. 
Acknowledgments 
We thank the crew of the RV Tommy Munro (Florida 
Fish and Wildlife Research Institute) and M. Murphy, B. 
Mahmoudi, and R. Lehnert for assistance in sampling, 
and C. Bradﬁeld and D. Ebelt for assistance in the labo-
ratory. Work was supported by the Marﬁn Program of 
the U.S. Department of Commerce (Grant NA04-NMF-
4330074), and by the Texas Agricultural Experiment 
Station (Project H-6703). This article is number 54 in 
the series “Genetic Studies in Marine Fishes” and is 
contribution number 147 of the Center for Biosystematics 
and Biodiversity at Texas A&M University. 
Literature cited 
Bagley, M. J., and J. B. Geller. 
1998. Characterization of microsatellite loci in the ver-
million snapper Rhomboplites aurorubens (Percoidei: 
Lutjanidae). Mol. Ecol. 7:1089−1090. 
Burton, M. L. 
2001. Age, growth, and mortality of gray snapper, Lut-
janus griseus, from the east coast of Florida. Fish. 
Bull. 99:254−265. 
Chamberlain, J. S., R. A. Gibbs, J. E. Ranier, P. N. Nguyen, and 
C. T. Caskey. 
1988.	 Deletion screening of the Duchenne muscular dys-
trophy locus via multiplex DNA amplification. Nucleic 
Acids Res. 16:11141−11156. 
Chistiakov, D. A., B. Hellemans, and F. A. M. Volckaert. 
2006. Microsatellites and their genomic distribution, evo-
lution, function and applications: a review with special 
reference to fish genetics. Aquaculture 255:1−29. 
Fischer, A. J., M. S. Baker Jr., C. A. Wilson, and D. L. Nieland. 
2005. Age, growth, mortality, and radiometric age 
validation of gray snapper (Lutjanus griseus) from 
Louisiana. Fish. Bull. 103:307−319. 
Gillig, D., W. L. Grifﬁn, and T. Ozuna Jr. 
2001. A bioeconomic assessment of Gulf of Mexico red 
snapper management policies. Trans. Am. Fish. Soc. 
130:117−129. 
Gold, J. R., E. Pak, and L. R. Richardson. 
2001. Microsatellite variation among red snapper (Lut-
janus campechanus) from the Gulf of Mexico. Mar. 
Biotechnol. 3:293−304. 
Neff, B. D., P. Fu, and M. R. Gross. 
2000. Microsatellite multiplexing in fish. Trans. Am. 
Fish. Soc. 129:584−593. 
Olsen, J. B., J. K. Wenburg, and P. Bentzen. 
1996. Semiautomated multilocus genotyping of Pacific 
salmon (Oncorhynchus spp.) using microsatellites. Mol. 
Mar. Biol. Biotechnol. 5:259−72. 
Renshaw, M. A., E. Saillant, S. C. Bradﬁeld, and J. R. Gold. 
2006. Microsatellite multiplex panels for genetic studies of 
three species of marine fishes: red drum (Sciaenops ocel-
latus), red snapper (Lutjanus campechanus), and cobia 
(Rachycentron canadum). Aquaculture 253:731−735. 
Rice, W. R. 
1989. Analyzing tables of statistical tests. Evolution 
43:223−225. 
Saillant, E., A. Fostier, P. Haffrey, B. Menu, J. Thimonier, and 
B. Chatain. 
2002. Temperature effects and genotype-temperature 
interactions on sex determination in the European 
sea bass (Dicentrarchus labrax L.). J. Exp. Zool. 
292:494−505. 
Saillant, E., and J. R. Gold. 
2006. Population structure and variance effective size 
of red snapper (Lutjanus campechanus) in the northern 
Gulf of Mexico. Fish. Bull. 104:136−148. 
Turner, T. F., J. P. Wares, and J. R. Gold. 
2002. Genetic effective size is three orders of magnitude 
smaller than adult census size in an abundant, estua-
rine-dependent marine fish (Sciaenops ocellatus). Ge-
netics 162:1329−1339. 
Van Oosterhout, C., W. F. Hutchinson, D. P. M. Willis, and 
P. Shipley. 
2004. MICRO-CHECKER: software for identifying and 
correcting genotyping errors in microsatellite data. Mol. 
Ecol. Notes 4:535−538. 
Wright, A. J., and P. Bentzen. 
1994. Microsatellites: genetic markers for the future. Rev. 
Fish Biol. Fish. 4:384−388. 


Microsatellite multiplex panels for genetic studies of gray snapper (Lutjanus griseus) and lane snapper (Lutjanus synagris)

http://aquaticcommons.org/8886/1/renshaw_Fish_Bull_2007.pdf

Microsatellite multiplex panels for genetic studies of gray snapper (Lutjanus griseus) and lane snapper (Lutjanus synagris)

Abstract

Similar works

Full text

Available Versions

Aquatic Commons