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CCLONES - ADEPT(Comparing Clonal Lines On Experimental Sites)
Forest Biology Research Cooperative
University of Florida
‘Series 1’ CCLONES Schedule
• Breeding 1996-1997• Sow seed March 2000• Top seedlings June 2000• Transplant seedling hedges Sept 2000• Randomize hedges on pad April 2001• Stick cuttings for rooting assessment1 May 2001• Stick cuttings for rooting assessment2 July 2001• Stick cuttings for Study B field tests Jan & May 2002• Screen 1400 clones for rust and PC 2002• Plant 915 clones on six locations December
2002• Measure phenotypes 2003
Breeding
• 30 top loblolly parents – Half from coastal plain; half from Florida
– “Good” for growth and rust, but variation among parents
• 70 full-sib families– Partial diallel with approx 4 to 5 crosses per parent
– Intent is to go to the field with 60 FS fams
Seed stratified: 1/24/00 Seed sown: 3/3/00
32 elite parents crossed in partial diallel to create ~2200 clones from 70 full-sib families
Study B seedlings after hedging (left) and prior to hedging (right) Seedlings were hedged in June 2000.
Hedged FBRC Study B seedlings 6 weeks after hedging.
Close-up of individual hedgesix weeks after hedging.
Close-up of individual hedge twelve weeks after hedging.
Hedges moved to 20,000 sq ft hedge-pad after transplanting
Experimental Design
– Randomization
• Clonal hedges were completely randomized on the hedge pad prior to setting
• Fixed-tray system (135 cells)
• Trays could then be randomized within each rep
Clonal hedges were randomized in April 2001.
‘Series 1’ CCLONES Schedule
• Sow seed March 2000• Top seedlings June 2000• Transplant seedling hedges Sept 2000• Randomize hedges on pad April 2001• Stick cuttings for rooting assessment1 May 2001• Stick cuttings for rooting assessment2 July 2001• Stick cuttings for Study B field tests Jan & May 2002• Screen 1400 clones for rust and PC 2002• Plant 915 clones on six locations December 2002• Measure phenotypes 2003
May 7, 2001-61 weeks after sowing
-46 weeks after initial topping of seedling
-11 weeks after last hedging
July
Shoot Collection
Preparing Cuttings To Set
30 Clones Per Tray
Typical Rooted Cutting(9 Weeks from setting)
Root AssessmentExperimental Design
– May 2001 setting
• Set ~2200 clones, 4 replications with 4-ramet row plots
• Assessed rooting 9 weeks after setting
• Counted # newly emerging roots from plug 9 weeks after setting
• Shoot dry weights obtained from 1 ramet per clone per rep (3 reps)
• Variance components estimated with ASREML
– July 2001 setting
• Set ~2200 clones, 5 replications with 4-ramet row plots
• Assessed rooting 9 weeks after setting
• Measured cutting diameter and height 9 weeks after setting (3 reps)
• Variance components estimated with ASREML
Summary of Rooting
Trial # of families # of clones# plots per
clone# cuttings per plot
Mean rooting %
Range of fam.
means
May 70 2194 4 4 54% 27-76%
July 70 2185 5 4 38% 18-69%
Variation Within Family for Rooting
0%10%20%30%40%50%60%70%80%90%
100%
Clone #
July
Roo
ting
%
Heritability Estimates For Root Number and Rooting %
0.00
0.05
0.10
0.15
0.20
0.25
0.30
0.35
Her
itab
ility
Root # May RT % July RT %
Trait Measured
DominanceAdditive
D/A = 0.16
D/A = 0.05
D/A = 0.14
64% rooting 81% rooting48% rooting
Differences in Shoot Morphology
Do these differences have an effect on rooting?
Differences in Root Morphology
‘Series 1’ CCLONES Schedule
• Breeding 1996-1997• Sow seed March 2000• Top seedlings June 2000• Transplant seedling hedges Sept 2000• Randomize hedges on pad April 2001• Stick cuttings for rooting assessment1 May 2001• Stick cuttings for rooting assessment2 July 2001• Stick cuttings for Study B field tests Jan & May 2002• Screen 1400 clones for rust and PC 2002• Plant 915 clones on six locations December
2002• Measure phenotypes 2003
Disease Screening
• 1400 clones from May and July setting sent to RSC– 22,000 rooted cuttings
– 5 to 20 ramets per clones
– Good rooting clones with approx equal numbers per family
• Four groups (with 5 or less ramets per clones)– Group 1: Rust with broad inoculum
– Group 2: Rust with narrow inoculum
– Group 3: PC with broad inoculum
– Group 4: PC with narrow inoculum
• Measure phenotypes (disease symptoms):– 1400 clones
– Two very different pathosytems
Resistance Screening at USFS - RSC
‘Series 1’ CCLONES Schedule
• Breeding 1996-1997• Sow seed March 2000• Top seedlings June 2000• Transplant seedling hedges Sept 2000• Randomize hedges on pad April 2001• Stick cuttings for rooting assessment1 May 2001• Stick cuttings for rooting assessment2 July 2001• Stick cuttings for Study B field tests Jan & May 2002• Screen 1400 clones for rust and PC 2002• Plant 915 clones on six locations December
2002• Measure phenotypes 2003
Field Locations
• Six Locations in FL and GA
• Design at each location:– 2 silvicultural treatments (HI and LO)
– 4 complete blocks per treatment
– Total of 8 ramets per clone (2 x 4) per site
– 915 clones from 60 FS families
– Total size approx 14 acres
– Total trees: 6 sites x 2 trts x 4 blocks x 915 clones = 44,000
• Two settings: Jan and April– Jan setting used for 3 sites
– April setting used for three sites
• Field planting in Dec 2002
Phenotyping of Association Pop’n• Rooting
– May and July 2001
– Jan and April 2002
• Disease symptoms– Rust and PC in RSC
– Rust in HI and LO treatments in field
• Standard growth:1, 2, 3 height in HI and LO
• Water deficit symptoms: 2 of 6 sites; 600 clones– Stable carbon isotopes at end of 1st season
– Specific leaf area
– Relative water content – two dry periods
– Water potential – two dry periods
• Other????
Acknowledgements
Forest Biology Research Cooperative
Special thanks to International Paper
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