USDA-ARS
refined pea core collection
for
26 quantitative traits
Coyne,
C.J.1, Brown, A.F.1,
1USDA-ARS, WRPIS,
Pullman
,
WA
,
USA
Timmerman-Vaughan,
G.M.2,
2Inst. for Crop and Food Res.,
Lincoln
,
New Zealand
McPhee,
K.E.3, and
3USDA-ARS, Grain Legume Genet. and Physiol.,
Pullman
,
WA
,
USA
Grusak,
M.A.4
4USDA-ARS, Children’s
Nutrition
Res.
Center
,
Houston
,
TX
,
USA
Introduction
Creation
of core subsets of crop germplasm collections was first suggested by Frankel (3)
as a way to efficiently utilize the genetic diversity present within the larger
collection. Ideally, core
collections represent the genetic diversity of a crop species and its wild
relatives (1). Core collections have
proven to be a successful way for plant scientists from many disciplines (plant
genetics, plant physiology, plant pathology) to first access a subset of
germplasm to help refine further exploration of the larger germplasm collection
held in trust in public institutions worldwide.
Among food legume crops distributed from the National Plant Germplasm
System (NPGS) repository located in Pullman, WA, USA, the pea core collection
(11) has been used frequently to screen for biotic stress resistance (4, 7), and
more recently for mineral nutrient analyses (5).
All data generated is publicly available through the Germplasm Resources
Information Network (GRIN) (http://www.ars-grin.gov/npgs/).
The
USDA-ARS Pisum germplasm collection
currently contains 3918 accessions. The first Pisum
core collection contained 504 accessions and inclusion was based on geographical
origin and flower color and was created using a proportional logarithm model to
determine number of accessions per country (geographic origin) (11).
Since establishment of the core collection, phenotypic data generated by
the repository and cooperators has been entered into the NPGS GRIN database by
cooperators. This refined core was created using biomass and related character
data (8), seed mineral nutrient composition (5), and seed protein concentration
(2). These data allow for the
application of multivariate statistical procedures such as cluster analysis to
understand the USDA pea core collection diversity for 26 quantitative traits.
The purpose of this study was to
investigate the possibility of reduce the size of the USDA pea core to
approximately 10% of the Pisum accessions using 26 quantitative traits
without reducing the trait diversity. Published
cores range in size from 5 to 20% of various crop germplasm collections using
passport, morphological and/or quantitative traits, typically a mixture of data
types (6). A recent example using
these three data types is for a chickpea core collection of accessions held in
India
(14). Given the core concept (3),
access to other and/or rare alleles is not diminished by whatever percent is
finally chosen as the USDA-ARS pea working collection remains the same at 3918
accessions. The 26 traits selected
were based on data availability for a significant portion of the USDA pea core
collection of some economically important characters of pea. The refined core
will be used for replicated field experiments and laboratory molecular studies
of allelic diversity of published pea genes and markers in the collection and to
begin to identify significant gaps in the core.
This baseline information on the refined pea core may contribute to
association mapping (linkage disequilibrium) studies in Pisum.
Materials
and methods
Plant
material and trait data
The
set of germplasm accessions used in this analysis was the USDA pea core
collection and they can be found http://www.ars-grin.gov/npgs/
under “Observations” and the descriptor “CORE” (11).
Quantitative data on 26 traits measured on the first core are listed
under their GRIN descriptor names, and published references are listed in Table
1. The pea core accessions and their
quantitative trait data used in this analysis are available at http://www.ars-grin.gov/npgs/
under “Observations”. Geographic
origin and flower color were not included in the analysis.
Table
1. Quantitative trait data used to reduce the size and redundancy in the USDA-ARS
pea core collection entered into the GRIN database (2,5,7).
|
Field
trait measurements
|
Number of accessions
|
Seed trait measurements
|
Number of accessions
|
|
Biomass (kg/ha)a
|
390
|
Cab
|
481
|
|
Seed yield (kg/ha) a
|
389
|
Mgb
|
481
|
|
Straw yield (kg/ha) a
|
389
|
Kb
|
481
|
|
Harvest index (yield/biomass) a
|
389
|
Pb
|
481
|
|
Days to first flower (50% with open
flowers) a
|
390
|
Feb
|
481
|
|
Days maturitya
|
390
|
Znb
|
481
|
|
Reproductive daysa
|
390
|
Mnb
|
481
|
|
Node to first flowera
|
390
|
Cub
|
481
|
|
Height to first flower nodea
|
390
|
Nib
|
481
|
|
Height at maturitya
|
390
|
Bb
|
458
|
|
Seed weight (g/100 seed) a
|
388
|
Mob
|
481
|
|
Seed & pod dry weight partitioning
(greenhouse) b
|
482
|
Seed positions (greenhouse) b
|
479
|
|
Seed dry weight (greenhouse) b
|
482
|
Seed protein concentration (greenhouse)
c
|
482
|
a
McPhee
and Muehlbauer, 2001.
b
Grusak
et al. 2004.
c
Coyne et al. 2005.
Statistical
methods
The
variables were standardized using the STAND module of NTSYSpc (9).
The linear transformation used is of the form:
y’= [(y-ŷ)/σ2y]-c
where
ŷ
= the mean of all y values, σ2y
= the standard deviation of all y values, and c = a constant added after the
above operations have been performed (9). Dissimilarity
coefficients for interval measure (quantitative) data were generated using the
SIMINT module of NTSYSpc. The
parameter of average taxonomic distance (DIST) module of NTSYSpc was used to
generate the matrix.
A
dendrogram was generated from the sequential, agglomerative, hierarchical, and
nested (SAHN) clustering method using the unweighted pair-group method
arithmetic average (UPGMA) (12) using the NTSYSpc SAHN module.
The
Euclid
coefficient (
EUCLID
module) was used to generate the dissimilarity matrix in Euclidean distances
for accessions in the new core. The
cut off point for the distance value of closely scored accessions based on the
26 trait measurements was set to result in a core of approximately 310
accessions. Random numbers were
assigned to accessions in the same cluster and used to select the accession from
each group for the refined core.
Comparison
of core collections
The
means of the original core and the refined core were compared for all 26 traits
using ANOVA (Proc GLM) and Tukey’s Studentized Range (HSD) modules of SAS
(10). The comparison of variances
between each of the 26 trait data of the original pea core with the refined pea
core was determined using ANOVA (Proc GLM) and Levene’s Test for homogeneity
of variances modules of SAS (10).
Results
and Discussion
The
purpose of this study was to investigate redundancy in the USDA pea core for 26
quantitative traits
and to use the relationships discovered to create a refined core for future
allelic diversity studies on economic
traits of pea. An underlying
assumption was that a core of 504 (~14%) selected in 1995 from the
approximately 3,500 pea accessions in the collection at that time may
over-represent the collection for these
26 quantitative traits. Additionally,
453 of the ~3500 accessions are Marx Genetic Stocks created by
backcrossing to the same parent, so the original core is closer to ~17% of the
1995 collection. Further
Table
2. Comparison
of means and variances between the original geographic core and the refined pea
core using 26 quantitative traits indicates that genetic diversity for these
traits was maintained (i.e., no significant loss of genetic variance in each
trait).
|
|
 Meansa
|
Variancesb
|
|
|
|
Traits
|
Original core
|
Refined core
|
α = 0.05
|
Original core
|
Refined core
|
F value
|
p
|
CV (%)c
|
Range (%)d
|
|
Biomass (kg/ha)
|
3330.1
|
3354.9
|
NSe
|
1132.5
|
1182.9
|
0.62
|
0.433
|
34.5
|
100
|
|
Seed yield (kg/ha)
|
1309.3
|
1308.7
|
NS
|
520.2
|
544.3
|
0.59
|
0.441
|
40.5
|
100
|
|
Straw yield (kg/ha)
|
2020.5
|
2045.8
|
NS
|
684.2
|
718.7
|
0.80
|
0.371
|
34.4
|
100
|
|
Harvest index
|
38.5
|
38.2
|
NS
|
7.0
|
7.5
|
0.72
|
0.395
|
18.8
|
100
|
|
Days to first flower
|
54.6
|
54.6
|
NS
|
5.8
|
5.9
|
0.14
|
0.704
|
10.7
|
100
|
|
Days to maturity
|
86.1
|
86.5
|
NS
|
9.8
|
9.9
|
0.21
|
0.643
|
11.4
|
100
|
|
Reproductive days
|
31.6
|
31.9
|
NS
|
7.5
|
7.7
|
0.23
|
0.634
|
23.9
|
100
|
|
Node first flower
|
15.3
|
15.2
|
NS
|
2.8
|
2.9
|
0.40
|
0.525
|
18.8
|
100
|
|
Height to first flower node
|
50.3
|
50.2
|
NS
|
15.1
|
15.7
|
0.57
|
0.452
|
30.5
|
100
|
|
Height at maturity
|
65.6
|
64.8
|
NS
|
18.4
|
18.8
|
0.14
|
0.705
|
28.4
|
96.5
|
|
Seed weight (g/100 seed)
|
16.2
|
16.3
|
NS
|
5.5
|
5.5
|
0.04
|
0.852
|
33.7
|
100
|
|
Seed & pod dw partitioning
|
88.0
|
88.1
|
NS
|
4.4
|
4.6
|
0.11
|
0.735
|
5.1
|
100
|
|
Seed dry weight
|
18.6
|
18.9
|
NS
|
7.4
|
7.4
|
0.02
|
0.886
|
39.5
|
100
|
|
Ca (ppm)
|
773.8
|
810.7
|
NS
|
321.0
|
359.9
|
2.06
|
0.152
|
42.7
|
100
|
|
Mg (ppm)
|
1693.5
|
1682.6
|
NS
|
168.9
|
183.2
|
1.19
|
0.276
|
10.3
|
100
|
|
K (ppm)
|
12622.5
|
12412.4
|
NS
|
1657.4
|
1673.2
|
0.02
|
0.887
|
13.2
|
100
|
|
P (ppm)
|
5163.6
|
5035.7
|
NS
|
953.8
|
999.2
|
0.87
|
0.350
|
19.0
|
100
|
|
Fe (ppm)
|
50.0
|
51.0
|
NS
|
11.7
|
12.1
|
0.35
|
0.552
|
23.5
|
91.7
|
|
Zn (ppm)
|
41.9
|
42.2
|
NS
|
11.5
|
11.7
|
0.07
|
0.798
|
27.5
|
100
|
|
Mn (ppm)
|
15.9
|
16.4
|
NS
|
4.5
|
4.8
|
0.28
|
0.594
|
28.8
|
100
|
|
Cu (ppm)
|
4.4
|
4.4
|
NS
|
1.7
|
1.8
|
0.21
|
0.646
|
39.4
|
100
|
|
Ni (ppm)
|
2.4
|
2.6
|
NS
|
1.6
|
1.8
|
0.64
|
0.426
|
69.0
|
100
|
|
B (ppm)
|
7.7
|
7.8
|
NS
|
1.6
|
1.6
|
0.14
|
0.709
|
20.3
|
100
|
|
Mo (ppm)
|
23.7
|
23.0
|
NS
|
8.4
|
8.0
|
1.00
|
0.319
|
35.2
|
82.9
|
|
Seed positions
|
5.7
|
5.7
|
NS
|
1.0
|
1.0
|
0.14
|
0.709
|
17.4
|
100
|
|
Seed protein concentration
(%)
|
24.1
|
24.0
|
NS
|
3.5
|
3.5
|
0.03
|
0.874
|
14.7
|
100
|
aDifferences
between means were tested by Tukey’s Studentized range test
(9).
bVariances
tested using Levene’s test for homogeneity (9).
cCV
= coefficient of variation calculated from ANOVA of the 26 traits between the
original core and the refined core.
d%
range was calculated from the minimum and maximum trait values of the original
core and the refined core.
eNS
= non-significant at the α
= 0.05 level (9).
phenotypic
and genotypic studies would need to be conducted to actually determine if this
is the case. The 310 accessions
included in the refined core collection are a subset of the 504 accessions in
the core collection. Comparison of
means and variances indicates no significant loss of genetic variation for 26
traits between the original core and the refined core (Table 2).
The dendogram of the refined USDA core collection can be found at http://www.ars-grin.gov/cgi-bin/npgs/html/eval.pl?492806,
under “Dendogram of the refined core (Power Point)”.
Interestingly,
Pisum sativum L. subsp. abyssinicum, known to be
very similar at the molecular level (13), was found grouped closely together
using these 26 quantitative traits. The
original USDA ARS core lacked representatives from Pisum
fulvum. We plan to add
accessions to fill this obvious gap in the refined core with Pisum
fulvum and to capture additional diversity of traits.
Since 1995, we have added over 400 new accessions, including subspecies
not in the 1995 collection from other germplasm collections and new plant
explorations to
Turkey
and central
Asia
. Examples of additional traits
identified would be accessions with improved resistance to Aphanomyces root rot
resistance (7) and Fusarium root rot (4). Additionally,
we plan to include accessions representing the extremes found for Mo (ppm) and
Fe (ppm) (Table 2). We are exploring
the core and refined core genetic diversity at the molecular level and will use
this information to further refine the USDA pea core collection.
As
Brown (1) predicted, “the composition of a core will change with time, as new
data, new material, or requirements come along”.
A core collection, especially a heavily used collection such as the
USDA pea core collection, will remain useful if it also remains dynamic.
Both the original USDA pea core and the refined pea core are found on the
GRIN web site under the Observations and Descriptors CORE and REFINED CORE (http://www.ars-grin.gov/npgs/).
Acknowledgments:
USDA-ARS Project 5348-21000-020-00 (Coyne) and USDA Foreign Agriculture
Service Project 5348-21000-020-03 (Coyne and Timmerman-Vaughan).
1. Brown, A.H.D. 1989.
In: Brown, A.H.D., Frankel, O.H.,
Marshall
, D.R. and Williams, J.T. (eds.) The
Use of Plant Genetic Resources.
Cambridge
University
Press,
Cambridge
,
UK
, pp 136-155.
2. Coyne, C.J., Grusak, M.A.,
Razai, L., and Baik, B.-K. 2005. Pisum
Genetics 37: XX-XX
3. Frankel, O.H. 1984.
In: Arber, W., Llimensee, K.,
Peacock, W.J. and Starlinger, P. (eds.) Genetic
Manipulations: Impact of Man and Society.
Cambridge
University
Press,
Cambridge
,
England
, pp 161–170.
4. Grünwald, N. J., Coffman,
V.A. and Kraft, J.M. 2003. Plant
Disease. 87: 1197-1200.
5. Grusak, M.A., Burgett, C.L.,
Knewtson, S.J.B., Lopéz-Millán, A.-F., Ellis, D.R., Li, C.-M., Musetti, V.M.,
and Blair, M.W. 2004. Proceedings
of the 5th AEP-2nd ICLGG Conference, pp 37-38.
6.
Johnson, R.C. and T. Hodgkin. 1999. Core
Collections for Today and Tomorrow. International
Plant Genet. Resources Inst.,
Rome
,
Italy
.
7. Malvick, D.K., and Percich,
JA. 1999. Plant
Disease 83: 51-54.
8. McPhee, K.E. and Muehlbauer,
F.J. 2001. Genetic
Res. Crop Evol. 48: 195-203.
9. Rohlf, F.J. 2000.
NTSYSpc: Numerical Taxonomy and
Multivariate Analysis System, version 2.11.
Exeter
Software, NY.
10.
SAS 9.1. 2002-2003. SAS
Institute,
Cary
,
NC
,
USA
.
11.
Simon, C.J. and Hannan, R.M. 1995.
HortScience 30: 907.
12.
Sneath, P.H.A. and Sokal, R.R. 1973.
Numerical Taxonomy. W.H.
Freeman and Co.,
San Francisco
,
USA
.
13.
Weeden, N.F. and Wolko, B. 2001.
Pisum Genetics 33: 21-25.
14.
Upadhyaya, H.D., Bramel, P.J., and Singh S. 2001.
Crop Sci 41: 206-210.