A Fast Air-dry Dropping Chromosome Preparation Method Suitable for FISH in Plants

Podsumowanie

A protocol is described for the preparation of high-quality mitotic plant chromosome spreads by a fast air-dry dropping method suitable for the FISH detection of single and high copy DNA probes.

Streszczenie

Preparation of chromosome spreads is a prerequisite for the successful performance of fluorescence in situ hybridization (FISH). Preparation of high quality plant chromosome spreads is challenging due to the rigid cell wall. One of the approved methods for the preparation of plant chromosomes is a so-called drop preparation, also known as drop-spreading or air-drying technique. Here, we present a protocol for the fast preparation of mitotic chromosome spreads suitable for the FISH detection of single and high copy DNA probes. This method is an improved variant of the air-dry drop method performed under a relative humidity of 50%-55%. This protocol comprises a reduced number of washing steps making its application easy, efficient and reproducible. Obvious benefits of this approach are well-spread, undamaged and numerous metaphase chromosomes serving as a perfect prerequisite for successful FISH analysis. Using this protocol we obtained high-quality chromosome spreads and reproducible FISH results for Hordeum vulgare, H. bulbosum, H. marinum, H. murinum, H. pubiflorum and Secale cereale.

Wprowadzenie

Fluorescence in situ hybridization (FISH) is an effective tool for the physical mapping of single and high copy sequences at the chromosomal level. Prerequisite is the preparation of high quality chromosome spreads. There is no general chromosome preparation protocol that would be equally suitable for animal and plant cells. Preparation of plant chromosomes is particularly challenging due to the rigid cell wall and various cytoplasm consistency within different species. One of the favorable methods for the preparation of plant chromosomes is a so-called drop technique also known as drop-spreading technique and air-drying technique ^1,2. This method was first introduced in 1958 by Rothfels and Siminovitch for in vitro grown mammalian cells ³. Later Martin et al. ⁴ and Kato et al. ⁵ adapted this method for plants.

More recently, a method named 'SteamDrop' was developed which used water steam for the preparation of non-overlapping chromosomes ⁶. Although, the positive influence of high humidity was observed earlier ⁷, 'SteamDrop' delivers a controlled workflow of high-quality chromosome preparations ⁶. The steam treatment causes stretching of chromosomes probably connected to some modifications of chromosomal proteins. The quality of resulting metaphase spreads is very high, although retaining of sufficient number of complete metaphase spreads for subsequent FISH experiments demands technical expertise.

Here we present a protocol for the preparation of mitotic cereal chromosomes suitable for the FISH detection of single and high copy probes ^5,8. This method is an improved variant of the air-dry dropping method described by Kato ⁹ performed under relative humidity of 50%-55% (Figure 1). This protocol comprises a reduced number of washing steps making its application easy, efficient and reproducible. Using this protocol we obtained high-quality chromosome spreads and FISH results for Hordeum vulgare, H. bulbosum, H. marinum, H. murinum, H. pubiflorum and Secale cereale.

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Protokół

1. Chromosome Preparation

1. Seed germination and fixation of root tips
   1. Germinate 10-20 barley seeds on two layers of moist filter paper in a Petri dish under dark conditions for 2 days at 22-24 °C. Cut off vigorous roots with the length of 1-2 cm from the seed by using a razor blade.
   2. Prepare ice-cold water by placing a 500 ml glass bottle containing cold tap water into crushed ice-water. Aerate the ice-cold water and immerse root tips for 20 hr to increase the frequency of metaphase cells.
   3. Transfer roots from water to 50 ml of ethanol: acetic acid (3:1) fixative to fix them at RT for 2 days. Store roots in a freshly prepared ethanol: acetic acid (3:1) fixative at 4 °C until use up to a year.
2. Washing and enzyme treatment
   1. Wash the 10-20 roots with 30 ml ice-cold tap water for 5 min twice using a 50 ml glass beaker. Use binocular microscope. Transfer roots one by one into 30 ml 0.01 M citrate buffer (0.01 M citric acid + 0.01 M sodium citrate, pH 4.8) using forceps and wash by shaking the glass beaker for 5 min twice. Place roots on filter paper to remove the liquid completely and cut-off undesired non-meristematic tissue using a razor blade.
   2. Incubate up to 20 root tips in 1 ml enzyme mixture at 37 °C for about 50 min to soften the plant tissue (Table 1) in a watch glass. Enzyme mixture contains 0.7% cellulase R10, 0.7% cellulase, 1% pectolyase and 1% cytohelicase diluted in 0.01 M citrate buffer. Store the enzyme mixture at -20 °C and reused up to five times.
   3. Remove the enzyme by pipetting and wash the root tips on ice with 5 ml 0.01 M citrate buffer twice to replace the residual enzyme.
3. Root maceration
   1. Wash root tips with 1 ml 96% ethanol twice carefully in the same watch glass. Replace ethanol with freshly prepared fixative (75% acetic acid : 25% ethanol). Use 10-15 µl fixative per root tip.
   2. Transfer root tips together with the fixative into a 2 ml tube and disintegrate root meristems with a dissecting needle or forceps. Tap the tube 20 times to re-suspend cells to obtain a cell suspension. Store the cell suspension at -20 °C up to two months.
4. Dropping of the cell suspension
   1. Place 2-3 layers of water-soaked paper tissue on a hot plate at 50 °C. Immerse microscopic slides in ice-cold tap water in the fridge for 30 min. And place slides on top of the moist paper tissue.
   2. Pipette 7-10 µl of cell suspension and drop it from a distance of 20 cm onto the cooled slide placed on the hot plate. Pipette 10 µl of acetic acid-ethanol mixture on the same place as cell suspension on the slide and keep the slide on the hot plate for additional 2 min. Place the slide on the hot plate without the wet tissue and let it dry for 1 min.
5. Quality control and storage of slides
   1. Check slides using a phase-contrast microscope to control the quality of the chromosome spread. Use slides either the same day or store by immersing in 96% ethanol in a Coplin jar at -20 °C.
6. Pretreatment of slides before FISH; all steps are carried out at RT
   1. Place slides in a Coplin jar containing 50 ml of 2x SSC (20x SSC contains 3 M NaCl and 300 mM trisodium citrate) for 5 min. Using forceps, transfer slides to a Coplin jar containing 50 ml of 45% acetic acid for 3-10 min.
   2. Transfer slides to a Coplin jar containing 50 ml of 2x SSC for 10 min. Transfer slides to a Coplin jar containing 50 ml of 4% formaldehyde (in 2x SSC) and immerse slides for 10 min to fix chromosomes.
   3. Remove formaldehyde by rinsing the slides 3 times for 4 min each, in a Coplin jar containing 50 ml 2x SSC. Dehydrate slides in a Coplin jar for 2 min in series of 70%, 90% and 100% ethanol, respectively and dry slides in a vertical position.

2. Fluorescent In Situ Hybridization (FISH)

1. For each slide, prepare a hybridization solution of 20 µl in total using 10 µl of deionized formamide, 5 µl of 4x hybridization buffer (200 µl buffer contains 80 µl 20x SSC, 8 µl 1 M Tris-HCl pH 8.0, 1.6 µl 0.5 M EDTA, 11.2 µl 10 µg/ µl salmon sperm and 99.2 µl DNase-free water), 3 µl of the probe and 2 µl of DNase-free water.
2. Add 20 µl of hybridization solution per slide and cover with a 24 x 32 mm cover slip and arrest the cover slip with rubber cement. Denature slides with probes simultaneously at 80 °C for 2 min on a hot plate.
3. Transfer slides to a moist chamber and incubate slides at 37 °C O/N avoiding light. Remove cover slips by rinsing the slides in a Coplin jar with 2x SSC. Place slides in a Coplin jar containing 55-60 °C 2x SSC and incubate for 20 min.
4. Place the slides to 2x SSC in a Coplin jar for 2 min at RT. Dehydrate slides in a Coplin jar for 2 min in series of 70%, 90% and 100% ethanol, respectively.
5. Air-dry the slides and counterstain with 1 µg/ml 4',6-diamidino-2-phenylindoline (DAPI) in antifade mounting medium, avoid intense light.

3. Microscopic Analysis and Storage

1. Analyze the slides using an epifluorescence microscope. The selection of filter depends on the fluorochrome used for probe labeling. If necessary, store slides at 4 °C under dark conditions up to a year.

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Wyniki

Microscopic slides with the mitotic metaphase spreads were prepared by the fast air-dry dropping chromosome preparation method described above (Suppl. Figure 1). FISH analysis was carried out using both, repetitive and single-copy sequences. Images were obtained by a epifluorescence microscope with a set of filters enabling excitation of corresponding fluorophores and captured by a high-sensitivity CCD monochrome camera. For the image acquisition we used a computer with an image acquisition software. Res...

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Dyskusje

The chromosome preparation experiment has been carried out using young roots of cereals belonging to the grass family (Poaceae). All analyzed species have 14 relatively long mitotic metaphase chromosomes (11-15 µm) in the diploid genome set and belong to large-genome species (5.1-7.9 Gbp).

Length of germinated roots was not more than 2 cm to obtain a maximum of meristematic tissue. Synchronization of dividing cells was achieved by a 20 hr long ice-water treatment that improved the quantit...

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Materiały

Name	Company	Catalog Number	Comments
Hot Plate	MEDAX GmbH	12603
Cellulase R10	Duchefa	C8001
Cellulase	CalBioChem	219466
Pectolyase	Sigma	P3026
Cytohelicase	Sigma	C8274
Texas Red-12-dUTP	Invitrogen	C3176	direct fluorochrome
Fluor488-5-dUTP	Invitrogen	C11397	direct fluorochrome
Fluorecsence microscope	Olympus BX61	BX61
CCD camera	Orca ER, Hamamatsu	C10600
4’,6-diamidino-2-phenylindole (DAPI)	Vector Laboratories	H-1200	fluorecsent dye