Establishing Pollination Requirements in Japanese Plum by Phenological Monitoring, Hand Pollinations, Fluorescence Microscopy and Molecular Genotyping

Brenda  I. Guerrero; Ma. Engracia Guerra; Javier Rodrigo

doi:10.3791/61897

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W tym Artykule

Podsumowanie
Streszczenie
Wprowadzenie
Protokół
Wyniki
Dyskusje
Ujawnienia
Podziękowania
Materiały
Odniesienia
Przedruki i uprawnienia

Podsumowanie

A methodology for the determination of pollination requirements in Japanese plum-type hybrids is described, which combines field- and laboratory-pollinations and observations of pollen tubes under the fluorescence microscopy with the identification of S-genotypes by PCR and the monitoring of flowering for the selection of pollinizers.

Streszczenie

The Japanese plum cultivars commonly grown are interspecific hybrids derived from crosses between the original Prunus salicina with other Prunus species. Most hybrids exhibit gametophytic self-incompatibility, which is controlled by a single and highly polymorphic S-locus that contains multiple alleles. Most cultivated hybrids are self-incompatible and need pollen from a compatible donor to fertilize their flowers. Establishing pollination requirements in Japanese plum is becoming increasingly important due to the high number of new cultivars with unknown pollination requirements. In this work, a methodology for the determination of pollination requirements in Japanese plum-type hybrids is described. Self-(in)compatibility is determined by hand-pollinations in both the field and in the laboratory, followed by monitoring pollen tube elongation with fluorescence microscopy, and also monitoring fruit maturation in the field. Selection of pollinizer cultivars is assessed by combining the identification of S-genotypes by PCR analysis with the monitoring of flowering time in the field. Knowing the pollination requirements of cultivars facilitates the selection of cultivars for the design of new orchards and allows the early detection of productivity problems related with pollination deficiency in established orchards.

Wprowadzenie

Japanese plum (Prunus salicina Lindl.) is native to China¹. In the 19^th century, this crop was introduced from Japan to the United States, where it was intercrossed with other North American diploid plums². In the 20^th century, some of these hybrids were spread to temperate regions around the world. Nowadays, the term “Japanese plum” refers to a wide range of interspecific hybrids derived from crosses between the original P. salicina with up to 15 other diploid Prunus spp.³^,⁴^,⁵.

Japanese plum, like other species of the Rosaceae family, exhibits Gametophytic Self-Incompatibility (GSI), which is controlled by a single and highly polymorphic S-locus containing multiple alleles⁶. The S-locus contains two genes that encode a ribonuclease (S-RNase) expressed in the pistil, and an F-box protein (SFB) expressed in the pollen grain⁷. In the self-Incompatibility reaction, when the S-allele expressed in the pollen grain (haploid) is the same as one of the two expressed in the pistil (diploid), the growth of the pollen tube across the style is arrested due to the degradation of the pollen tube RNA by the action of the S-RNase⁸. Since this process prevents fertilization of the female gametophyte in the ovule, GSI promotes the outcrossing between cultivars.

Although some Japanese plum cultivars are self-compatible, most cultivars currently grown are self-incompatible, and need pollen from inter-compatible donors to fertilize their flowers³. In stone fruit species of genus Prunus such as almond⁹, apricot¹⁰^,¹¹^,¹² and sweet cherry¹³, pollination requirements of cultivars can be established by different approaches. Self-(in)compatibility can be determined by self-pollination of flowers in the field and subsequent monitoring of fruit set, or by semi-in vivo self-pollinations at controlled conditions in a laboratory and the observation of pollen tubes under the microscope¹⁴^,¹⁵^,¹⁶^,¹⁷^,¹⁸. Incompatibility relationships among cultivars can be determined by cross pollinations in the field or the laboratory using pollen of the potential pollinizer cultivar, and by the identification of S-alleles of each cultivar by PCR analysis¹⁴^,¹⁵^,¹⁶^,¹⁹^,²⁰^,²¹^,²². In species such as sweet cherry or almond, self-(in)compatibility can be also assessed by the identification of particular S alleles associated to self-compatibility, as S₄’ in sweet cherry¹³ or S_f in almond²³.

Several plum breeding programs from the main producing countries are releasing a number of new cultivars²^,¹⁴, many of them with unknown pollination requirements. In this work, a methodology for the determination of pollination requirements in Japanese plum-type hybrids is described. Self-(in)compatibility is determined by self-pollinations in both the field and the laboratory, followed by observations of pollen tubes under the fluorescence microscopy. Selection of pollinizer cultivars combines the identification of S-genotypes by PCR analysis with the monitoring of flowering time in the field.

Protokół

1. Hand-pollination in the field

Pollen extraction
1. To obtain pollen, collect flower buds at stage D²⁴, according to stage 57 on the BBCH scale²⁵^,²⁶.
  NOTE: More flower buds are necessary in Japanese plum than in other Prunus species because their anthers produce less pollen.
2. Remove the anthers using a plastic mesh (2 mm x 2 mm pore size) and place them on paper at room temperature for 24 h until anther dehiscence.
3. Sieve the pollen grains through a fine mesh (0.26 mm x 0.26 mm pore size), and conserve them in a 10 mL glass tube with a cap at 4 °C until use.
Pollination of emasculated flowers
1. When between 10%–20% of flowers are open, select and label several branches. Remove open flowers and young buds, leaving only flower buds at stage D²⁴, according to stage 57 on the BBCH scale²⁵^,²⁶.
2. Remove the petals, sepals, and stamens of between 800 and 1,000 flower buds per treatment with either fingernails or tweezers.
3. Hand pollinate the pistils with the help of a fine paintbrush 24 h after emasculation. Some branches containing half of the pistils with pollen of the same cultivar, and the other half with compatible pollen from other cultivar as a control. Be careful not to contaminate the fingertip or paintbrush with pollen grains from other cultivars.
4. Record weekly counts of flowers and developing fruits to characterize fruit drop pattern and quantify the final fruit set in each pollination treatment.
Supplementary pollination in the field
1. A few days before the first flowers open, enclose selected trees in a 0.8 mm mesh cage to avoid the arrival of pollinating insects.
2. When 10%–20% flowers are open, select and label several branches per pollination treatment, leaving 1,000–1,500 flowers per treatment.
3. On the next day, when flowers are open, pollinate each flower with the help of a paintbrush with the corresponding pollen (pollen from the same cultivar for self-pollination, and from other compatible cultivars as cross-pollination control).
4. Pollinate every other day until all flowers open.
5. Record weekly counts of flowers and developing fruits from anthesis to harvest to characterize fruit drop pattern and quantify final fruit set in each pollination treatment.

2. Hand-pollinations in the laboratory

Collect 50–100 flowers at stage D²⁴, according to stage 57 on the BBCH scale²⁵^,²⁶.
In the laboratory, emasculate 30 flowers per treatment (self- and cross-pollination).
NOTE: Emasculation should be proceeded carefully to avoid any damage on the pistils.
Make a fresh cut on the base of each flower pedicel underwater before placing it on a piece of wet florist foam (one piece of foam for each pollination treatment).
Hand pollinate each pistil 24 h later using a fine paintbrush with pollen collected previously (see section 1.1). Pollinate one set of pistils with pollen from the same cultivar, and the other set with pollen from a compatible cultivar as control.
Leave the pollinated pistils 72 h after pollination at room temperature. The floral foam should be continuously wet with water.
Fix the pistils in a fixative solution of ethanol/acetic acid (3:1) for at least 24 h at 4 °C. Replace the fixative with 75% ethanol. Samples can be conserved in this solution at 4 °C until use²⁷.
NOTE: Ensure that the samples are completely submerged in the solution.

3. Microscopic observations

Evaluation of in vitro pollen germination
1. To elaborate pollen germination medium, dissolve 25 g of sucrose on 250 mL of distilled water, then add 0.075 g of calcium nitrate [Ca(NO₃)₂] and 0.075 g of boric acid (H₃BO₃).
2. Add 2 g of agar to the solution and mix until completely dissolved²⁸.
3. To sterilize the medium, autoclave it at 120 °C for 20 min. Cool the medium and, before it solidifies, distribute 3 mL per sterile Petri dish (55 mm x 12 mm) in a sterile laminar flow hood. After medium solidification, conserve the Petri dishes wrapped in aluminum foil at 4 °C until use.
4. Spread the pollen of each cultivar previously used as pollen donor in the controlled pollinations in two Petri dishes and incubate them at 25 °C for 24 h.
  NOTE: The inoculated culture media can be observed with microscopy immediately after or stored at -20 °C until use. For this purpose, the Petri dishes should be changed from the freezer to the fridge 24 h before microscopy observations.
5. To observe the pollen grains, prepare 1% (v/v) aniline blue solution that stains callose. First, prepare a 0.1 N potassium phosphate tribasic (K₃PO₄) solution by dissolving 7.97 g of K₃PO₄ in 1,000 mL of distilled water. To elaborate the 1% (v/v) aniline blue solution, dissolve 1 mL of aniline blue in 100 mL of 0.1 N K₃PO₄.
6. Add 2–3 drops of aniline blue solution to each Petri dish plate and observe after 5 min under a UV epifluorescence microscope using exciter filter BP340-390 and barrier filter LP425. Count viable and non-viable pollen grains in three fields per plate, each field containing 100-200 pollen grains, in two Petri dishes for each cultivar.
Pollen tube growth
1. Rinse the fixed pistils with distilled water three times (1 h each, 3 h in total) and transfer to 5% (w/v) sodium sulphite (Na₂SO₃) at 4 °C for 24 h. To prepare this solution, dissolve 5 g of sodium sulphite in 100 mL of distilled water.
2. Autoclave the pistils at 120 °C for 8 min in 5% (w/v) sodium sulphite to soften the tissues.
3. Squash softened pistils in a drop of 1% (v/v) aniline blue solution under a cover glass on a slide to stain callose.
4. Observe pollen tube growth along the style under a microscope with UV epifluorescence using exciter filter BP340-390 and barrier filter LP425.

4. Determining incompatibility relationships

DNA extraction from leaves
1. To extract DNA, collect 3–4 young leaves of each cultivar in the field, preferably in spring.
  NOTE: DNA can also be extracted from mature leaves, but DNA from young leaves has less phenolic compounds.
2. Isolate DNA using a commercial kit and follow the provided protocol kit (see Table of Materials).
3. Quantify the DNA concentration and evaluate the quality of the DNA of each sample at 260 nm in an UV-Vis microvolume spectrophotometer. Adjust the DNA concentration to 10 ng/μL.
PCR conditions for fragment amplification
1. Label 0.2 mL PCR tubes and caps.
2. Prepare the PCR reagents according to Table 1 and let them thaw on ice.
3. Set up a volume of master mix of each pair of primers in a 1.5 mL microtube according to the number of reactions plus 10% of excess, considering a volume of 16 μL per reaction. Add the reagents following the order in Table 1 and mix thoroughly.
4. Aliquot 16 μL of master mix into each 0.2 mL PCR tube containing 4 μL of DNA template or 4 μL of sterilized distilled water as negative control (C-). Use DNA of cultivars with known genotype as positive controls. Mix gently, close the reaction tubes with the caps, and centrifugate at 2,000 x g for 30 s to collect the entire volume at the bottom of the reaction tube.
5. Place the reaction tubes in the thermocycler and set up the PCR program using the following temperature profile: an initial step of 3 min at 94 °C, 35 cycles of 1 min at 94 °C, 1 min at 56 °C and 3 min at 72 °C, and a final step of 7 min at 72 °C²⁰.
Electrophoresis and estimation of fragment size
1. To prepare a 1.7% (w/v) agarose mini gel, dissolve 0.68 g of agarose and 40 mL of 1x TBE buffer into a 100 mL Erlenmeyer flask. Melt the solution by heating in a microwave at 600 W at 30 s intervals to avoid boiling.
2. Let the solution stay on the bench to cool down, and then add 3.5 μL of nucleic acid staining solution.
3. Place the gel tray into the casting stand and put the selected comb into the gel mold. Be sure to have enough wells for each PCR product and DNA ladder.
4. Pour the agarose solution into the gel mold and let it cool down until polymerization. Remove the comb of the polymerized gel. Place the gel in the horizontal electrophoresis system containing enough 1x TBE buffer to cover the surface of the gel.
5. Load the first and last wells with 2 μL of the DNA molecular weight ladder (1 kb DNA Ladder). Load 3 μL of each product of the PCR in the other wells. Close the chamber, turn on the power, and run the gel at 100 V for 30 min.
6. Observe the gel under UV light using a gel documentation system. Use the DNA molecular weight ladder to determine the size of the amplified fragment and compare it with the positive controls in order to identify the corresponding alleles.

5. Monitoring flower dates

Monitor the phenology of different trees of each cultivar at flowering over different years. Establish the length of the flowering period from the first (about 5%) to the last open flowers (about 95%). Full bloom is considered when at least 50% of flowers are at stage F²⁴, according to stage 65 on the BBCH scale²⁵^,²⁶.
To compare the flowering dates of inter-compatible cultivars and determine those that coincide at flowering time every year, elaborate a calendar of flowering times with data from several years.

Wyniki

Each Japanese plum flower bud contains an inflorescence with 1–3 flowers. As in other stone fruit species, each flower is made up of four whorls: carpel, stamens, petals, and sepals, which are fused forming a cup at the base of the flower. Flower structures are smaller than other stone fruits, with a short and fragile pistil surrounded by the stamens that contain a small amount of pollen grains. At full bloom, the flowers of each inflorescence appear separated on short stalks, showing the white petals forming a bal...

Dyskusje

The methodology described herein for pollination requirements of Japanese plum cultivars requires determining the self-(in)compatibility of each cultivar by controlled pollinations in the field or the laboratory, and the subsequent observation of pollen tube growth with fluorescence microscopy. The incompatibility relationships are established by the characterization of the S-alleles by molecular genotyping. Finally, the selection of pollinizers is performed by the monitoring phenology to detect those cultivars ...

Ujawnienia

The authors have nothing to disclose.

Podziękowania

This research was funded by Instituto Nacional de Investigación y Tecnología Agraria y Alimentaria (RFP2015-00015-00 and RTA2017-00003-00); Gobierno de Aragón—European Social Fund, European Union (Grupo Consolidado A12-17R), and Junta de Extremadura —Fondo Europeo de Desarrollo Regional (FEDER), Plan Regional de Investigación (IB16181), Grupo de Investigación (AGA001, GR18196). B.I. Guerrero was supported by a fellowship of Consejo Nacional de Ciencia y Tecnología of México (CONACYT, 471839).

Materiały

Name	Company	Catalog Number	Comments
Acetic Acid Glacial	Panreac	131008.1611
Agar	iNtRON Biotechnology	25999
Aniline blue	Difco	8504-88
Boric Acid (H₃BO₄)	Panreac	131015.1210
Calcium Nitrate 4-hydrate (Ca(NO₃)₂·4H₂O)	Panreac	131231.1211
Coverglass	Deltalab	D102460	24 mm x 60 mm
Digital Camera	Imaging Developmet Systems	UI-1490SE
Digital Camera Software Suite	Imaging Developmet Systems	4.93.0.
DNA Oligos	ThermoFisher Scientific
dNTP Mix, 10 mM each	ThermoSischer Scientific	R0193
DreamTaq Green DNA polymerase	ThermoFisher Scientific	EP0713
Ethanol 96°	VWR-Chemicals	83804.360
1Kb DNA Ladder (U.S. Patent No. 4.403.036) (500pb-12Kb)	Invitrogen	15615-016	Size: 250µg; Conc: 1.0 µg/µl
Gel Documentation System	Bio-Rad	1708195
Hand Counter	Tamaco	TM-4
Image Lab Software	Bio-Rad		Image Analyse System for Gel Documentation System
MetaPhor Agarose	Lonza	50180
Microcentrifuge 5415 R	Eppendorf	Z605212
Microscope with UV epiflurescence	Leica	DM2500	Exciter filter BP340-390, Barrier filter LP425
Microslides	Deltalab	D100004	26 mm x 76 mm
Mini Electrophoresis System	Fisherbrand	14955170
Minicentrifuge	ThermoFisher Scientific	15334204
NanoDrop 1000 Spectrophotometer	ThermoFisher Scientific	ND1000
Petri Dishes	Deltalab	200201	55 mm x 14 mm
Potassium Phosphate Tribasic (K₃PO₄·1.5H₂O)	Panreac	141513
Primer forward 'Pru C2'	ThermoFisher Scientific
Primer forward Pru T2'	ThermoFisher Scientific
Primer reverse 'PCER'	ThermoFisher Scientific
RedSafe Nucleic Acid Staining Solution	iNtRON Biotechnology	21141
Saccharose	Panreac	131621.1211
Sodium sulphite anhydrous (Na₂SO₃)	Panreac	131717.1211
Speedtools plant DNA extraction Kit	Biotools	21272
TBE Buffer (10X)	Panreac	A0972,5000PE
Thermal Cycler T100	Bio-Rad	1861096
Thermomixer comfort	Eppendorf	T1317
Vertical Autoclave Presoclave II	JP Selecta	4001725
Vortex	Fisherbrand	11746744

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