Summary

Polysome Purification from Soybean Symbiotic Nodules

Published: July 01, 2022
doi:

Summary

This protocol describes a method for eukaryotic polysome purification from intact soybean nodules. After sequencing, standard pipelines for gene expression analysis can be used to identify differentially expressed genes at the transcriptome and translatome levels.

Abstract

The aim of this protocol is to provide a strategy for studying the eukaryotic translatome of the soybean (Glycine max) symbiotic nodule. This paper describes methods optimized to isolate plant-derived polyribosomes and their associated mRNAs to be analyzed using RNA-sequencing. First, cytoplasmic lysates are obtained through homogenization in polysome- and RNA-preserving conditions from whole, frozen soybean nodules. Then, lysates are cleared by low-speed centrifugation, and 15% of the supernatant is used for total RNA (TOTAL) isolation. The remaining cleared lysate is used to isolate polysomes by ultracentrifugation through a two-layer sucrose cushion (12% and 33.5%). Polysome-associated mRNA (PAR) is purified from polysomal pellets after resuspension. Both TOTAL and PAR are evaluated by highly sensitive capillary electrophoresis to meet the quality standards of sequencing libraries for RNA-seq. As an example of a downstream application, after sequencing, standard pipelines for gene expression analysis can be used to obtain differentially expressed genes at the transcriptome and translatome levels. In summary, this method, in combination with RNA-seq, allows the study of the translational regulation of eukaryotic mRNAs in a complex tissue such as the symbiotic nodule.

Introduction

Leguminous plants, such as soybean (Glycine max), can establish symbiosis with specific soil bacteria called rhizobia. This mutualistic relationship elicits the formation of novel organs, the symbiotic nodules, on the plant roots. The nodules are the plant organs hosting the bacteria and consist of host cells whose cytoplasm is colonized with a specialized form of rhizobia called bacteroids. These bacteroids catalyze the reduction of atmospheric nitrogen (N2) into ammonia, which is transferred to the plant in return for carbohydrates1,2.

Although this nitrogen-fixing symbiosis is one of the most well-studied plant-microbe symbioses, many aspects remain to be better understood, such as how plants subjected to different abiotic stress conditions modulate their interaction with their symbiotic partner and how this affects nodule metabolism. These processes could be better understood by analyzing the nodule translatome (i.e., the subset of messenger RNAs [mRNAs] actively translated). Polyribosomes or polysomes are complexes of multiple ribosomes associated with mRNA, commonly used to study translation3. The polysome profiling method consists of the analysis of the mRNAs associated with polysomes and has been successfully used to study the posttranscriptional mechanisms controlling gene expression that occurs in diverse biological processes4,5.

Historically, genome expression analysis has focused primarily on determining mRNA abundance6,7,8,9. However, there is a lack of correlation between transcript and protein levels due to the different stages of posttranscriptional regulation of gene expression, particularly translation10,11,12. Moreover, no dependence has been observed between the changes at the level of the transcriptome and those that occur at the level of the translatome13. The direct analysis of the set of mRNAs that are being translated allows a more accurate and complete measurement of the cell gene expression (whose endpoint is protein abundance) than the one obtained when only mRNA levels are analyzed14,15,16.

This protocol describes how plant-derived polysomes are purified from intact soybean nodules by differential centrifugation through a two-layer sucrose cushion (Figure 1). However, since bacteroid-derived ribosomes are also present in the nodules, a mix of ribosomes and RNA species are purified, even though the eukaryotic ones represent the main fraction (90%-95%). The subsequent RNA isolation, quantification, and quality control are also described (Figure 1). This protocol, in combination with RNA-seq, should provide experimental results on the translational regulation of eukaryotic mRNAs in a complex tissue such as the symbiotic nodule.

Figure 1
Figure 1: Schematic overview of the proposed methodology for eukaryotic polysome purification from symbiotic nodules. The scheme gives an overview of the steps followed in the protocol from (1) plant growth and (2) nodule harvest to (3) preparation of the cytosolic extracts, (3) obtaining TOTAL samples and (4) PAR samples, and (5) RNA extraction and quality control. Abbreviations: PEB = polysome extraction buffer; RB = resuspension buffer; TOTAL = total RNA; PAR = polysome-associated mRNA. Please click here to view a larger version of this figure.

Protocol

1. Plant growth and rhizobia inoculation

  1. To generate the required nodules, sow the soybean seeds of choice in the selected substrate in a growth chamber under controlled conditions.
    NOTE: In this protocol, seeds were sown in a 0.5 L plastic bottle filled with a mix of sand:vermiculite (1:1). The growth chamber was set with a day/night cycle temperature of 28 °C /20 °C, respectively, and a light/darkness photoperiod of 16 h/8 h, respectively. The photosynthetically active radiation intensity was 620 µmol·m−2·s−1.
  2. Prepare in advance liquid Yeast-Extract Mannitol (YEM)-medium (see the Table of Materials). Autoclave the medium.
  3. On the same day of seed sowing, inoculate one flask containing 100 mL of YEM with the Bradyrhizobium elkanii U1302 strain. Incubate the flask at 28 °C on an orbital shaker at 100 rpm.
    1. Let the rhizobia grow for 2 days and inoculate the seedlings with 2 mL of the culture.

2. Water deficit treatment (optional)

NOTE: This protocol outlines the water deficit treatment of the soybean plants. This part can be changed or omitted entirely depending on the experimental question at hand.

  1. Grow the soybean seedlings for 19 days (V2-3 developmental stage) without water restriction. Keep the substrate at field capacity with B&D-medium17 supplemented with 0.5 mM KNO3.
  2. On day 20, withdraw watering.
    NOTE: Here, the water content was measured daily by gravimetry (water gravimetric content) during the growth and water deficit periods.
  3. Measure stomatal conductance in triplicate daily on the abaxial leaf surface with a porometer, as instructed by the manufacturer (see the Table of Materials), from day 20 until the end of the water deficit period.
    ​NOTE: The end of the water deficit period was determined individually for each plant when the stomatal conductance value was approximately 50% of the one obtained on day 20 from sowing.

3. Nodule harvest

  1. Collect liquid nitrogen in a clean container and label 15 mL tubes (one for each plant).
    CAUTION: Handle liquid nitrogen wearing cryo gloves, face shields, and safety goggles.
  2. Retrieve each plant individually. Cut and discard the aerial part. Thoroughly wash the root with water to remove any remaining substrate.
  3. Detach each nodule from the root and collect them in a prechilled 15 mL tube. Snap-freeze the tubes and store them at −80 °C.

4. Preparation of cytosolic extracts

NOTE: The final aim of this protocol is to obtain high-quality total RNA (TOTAL) and polysome-associated RNA (PAR). Therefore, work under conditions that prevent RNA degradation, always keeping the samples at 4 °C and using RNase-free laboratory equipment and solutions. Unless specified, all the solutions are prepared with sterile ultrapure water.

  1. Preparation of buffer stock solutions
    1. Prepare the autoclavable stock solutions listed in Table 1, autoclave them for 15 min, and keep at RT.
    2. Prepare the filter-sterilizable stock solutions listed in Table 1, filter-sterilize them, and keep them at −20 °C.
  2. Prepare polysome extraction buffer (PEB, see Table 1) and keep it on ice.
    NOTE: The volumes given are for six samples.
  3. Cool the centrifuge to 4 °C and place 2 mL microcentrifuge tubes on ice.
  4. Weigh approximately 0.2 g of intact nodules in a weighing dish and transfer them to a precooled 2 mL tube.
    NOTE: Perform this step quickly to avoid the thawing of the samples. Alternatively, an estimated nodule volume of 0.4-0.5 mL can be used instead of the 0.2 g.
  5. Add 1.2 mL of PEB, let the sample thaw for 2 min, and homogenize with a tissue grinder until complete disruption and homogenization of the nodules.
    NOTE: Be sure to grind the nodules once thawed as they will be soft enough to be easily disrupted with tissue grinders (see the Table of Materials) in microcentrifuge tubes. Frozen nodules are difficult to grind. Also, it is recommended to place the tubes in a benchtop cooler (0 °C) for proper homogenization while keeping samples cool.
  6. Incubate the samples on ice with gentle agitation for 10 min or until all samples have been processed.
  7. Centrifuge at 16,000 × g for 15 min at 4 °C to pellet the debris. Recover the supernatant and repeat the centrifuge step.
  8. Carefully recover the clarified cytosolic extract and transfer a 200 µL aliquot to a clean 1.5 mL microcentrifuge tube for TOTAL isolation (TOTAL samples; see section 7).

5. Preparation of sucrose cushions

NOTE: This protocol uses a two-layer sucrose cushion (12% and 33.5%) in 13.2 mL ultracentrifuge tubes (see the Table of Materials). All solutions are prepared with sterile ultrapure water.

  1. Prepare the sucrose and salt stock solutions.
    1. Prepare 100 mL of 2 M sucrose solution (68.5%, Table 1).
    2. Prepare 10x salt solution (Table 1).
  2. Prepare the two layers of the sucrose cushion as described in Table 2. See Table 1 for the composition of the antibiotic (CHX and CHL) stock solutions.
    NOTE: The volumes given are for six cushions.
  3. Pour 4.5 mL of the 33.5% sucrose layer into the centrifuge tubes. Then, add 4.5 mL of the 12% layer carefully and slowly with a P1000 micropipette. Put the tubes on ice until the addition of the clarified cytosolic extract.

6. Polysome purification

  1. Load 1 mL of the clarified cytosolic extract (step 4.8) on top of the sucrose cushion by carefully pipetting onto the sidewall of the tube.
  2. Transfer the ultracentrifuge tubes to precooled buckets and centrifuge at 217,874 × g (35,000 rpm in the referenced rotor [see the Table of Materials]) for 2 h at 4 °C.
  3. Discard the remaining cytosolic extract and sucrose cushion, and resuspend the polysomal pellet with 200 µL of precooled RB (previously prepared according to Table 1).
  4. Incubate for 30 min on ice and then transfer the polysomal resuspension to 1.5 mL precooled tubes. Proceed with the RNA extraction (PAR samples).

7. RNA extraction and quality control

NOTE: This step is performed for TOTAL (step 4.8) and PAR samples (step 6.4).

  1. Prepare 75% EtOH with sterile ultrapure water and cool it to −20 °C. Additionally, cool chloroform and isopropanol to −20 °C.
  2. Homogenize the samples with 750 µL of the RNA isolation reagent and incubate for 5 min at RT.
  3. Add 200 µL of cold chloroform and shake the tubes vigorously for 15 s. Incubate at RT for 10 min.
  4. Centrifuge at 12,000 × g for 15 min at 4 °C for phase separation. Transfer 500 µL of the upper aqueous phase to a clean tube without disturbing the pink organic phase, and add 375 µL of cold isopropanol and 0.5 µL of RNase-free glycogen (see the Table of Materials). Mix thoroughly by pipetting up and down.
    NOTE: Glycogen is a carrier used as a co-precipitant to increase nucleic acid recovery from alcohol precipitation.
  5. Incubate the mix for 10 min at 4 °C and centrifuge at 12,000 × g for 15 min. Discard the supernatant.
  6. Wash the RNA precipitate with 1 mL of cold 75% EtOH. Mix by brief vortexing.
    NOTE: At this point, the samples can be stored at −20 °C overnight.
  7. Centrifuge at 7,500 × g for 5 min at 4 °C, carefully remove the supernatant with a micropipette, and air-dry the RNA pellet.
  8. Dissolve the pellet in 50 µL of RNase-free water and incubate at 65 °C for 5 min.
  9. Assess the RNA concentration and integrity with highly sensitive capillary electrophoresis18 (see the Table of Materials) and/or electrophoresis on a 2% RNase-free agarose gel19 (see the Table of Materials).
    NOTE: If the RNA samples are not going to be used immediately or are going to be sent to the sequencing facility for RNA-seq library preparation, it is recommended to use EtOH to precipitate them.

8. RNA precipitation

  1. Cool the centrifuge and EtOH to 4 °C.
  2. Prepare 3 M sodium acetate.
  3. Prepare 70% EtOH with sterile ultrapure water and cool it to −20 °C.
  4. Estimate the sample volume. Add 0.1 volumes of 3 M sodium acetate, 3 volumes of cold EtOH, and 0.5 µL of RNase-free glycogen. Mix thoroughly.
  5. Leave at −20 °C until needed.
    ​NOTE: RNA precipitated samples can be stored for up to 1 year at −80 °C.

9. Standard pipeline for gene expression analysis

  1. Perform an average of 40M Illumina paired-end reads, with read length >100 bp, for confident transcriptome and translatome data analysis.
    NOTE: Standard RNA-seq data analysis includes the following steps 9.2-9.5.
  2. Carry out read quality inspection using FastQC (https://www.bioinformatics.babraham.ac.uk/projects/fastqc/) or the multisample MultiQC20.
  3. Remove adaptor and low-quality sequences using either Trimmomatic21, BBDuk (http://jgi.doe.gov/data-and-tools/bb-tools/), cutadapt22, sickle23, or Trim Galore (https://www.bioinformatics.babraham.ac.uk/projects/trim_galore/), among others.
  4. If a reference genome is available for the species, carry out read mapping against the reference, followed by abundance quantification, using Bowtie224, TopHat225 or Salmon26, and featureCounts27, besides other open source tools.
  5. Perform statistical analysis for differential expressed genes identification using edgeR28, DESeq229, or limma30, among others.
    NOTE: These open-source software can be used locally, via the command line. Alternatively, they can be operated through a web browser on a public server, such as Galaxy31 or GEOexplorer32, which offer a graphical user interface, so that no command line knowledge is required for their use.

Representative Results

The quantity and quality assessment of the TOTAL and PAR fractions purified with the abovementioned procedure is key to determining its success, since for most downstream applications, such as RNA sequencing, high-quality samples are fundamental for library preparation and sequencing. Moreover, the integrity of the RNA molecules allows the capture of a snapshot of the gene expression profile at the moment of sample collection18. In this context, an RNA integrity number (RIN) is obtained when performing these measurements using a Bioanalyzer. The RIN is used for assigning integrity values in a robust, reliable, and user-independent way, ranging from 10 (intact) to 1 (totally degraded)18.

Figure 2A,B show the standard output of the high-sensitivity capillary electrophoresis system (Bioanalyzer) for several TOTAL and PAR sample fractions. Very good quality is observed for all the samples since sharp ribosomal RNA (rRNA) bands can be visualized without any smeared appearance. However, this is not reflected in the RIN values, as they range between 5.9 and 7.5, which corresponds to non-intact samples. Nevertheless, as previously mentioned, there is no visual sign of sample degradation, as can be seen in Figure 2C. Figure 2D shows an example of a bioanalyzer result of an almost entirely degraded sample for comparison. The equipment also failed to identify the 18S and 25S peaks, as seen in the electropherograms both for TOTAL and PAR samples (Figure 2B). Consequently, the proportion of the ribosomal bands (25S:18S; another indicator of RNA integrity) could not be calculated. High-quality RNA usually exhibits a 25S:18S 2:1 ratio33.

Figure 2
Figure 2: Total RNA and polysome-associated mRNA quantity and quality assessment. (A) Representative virtual gel reconstruction of high-sensitivity capillary electrophoresis (Bioanalyzer) results from 12 samples with their respective RIN and concentration values. Lane 1 to lane 6 correspond to total RNA (TOTAL) fractions of six nodule samples, and lane 7 to lane 12 correspond to polysome-associated mRNA (PAR) fractions of the same samples. Green line: lower marker present in all lanes. (B) Electropherogram representation is shown for sample 4 (as an example of TOTAL) and sample 10 (as an example of PAR). 18S and 25S peaks are indicated. Peaks possibly corresponding to 16S and 23S (prokaryotic rRNAs) are indicated with *. Zoom-ins on these peaks are shown (B1 and B2). The Eukaryote Total RNA Nano assay was used in the Bioanalyzer. (C) Representative agarose gel electrophoresis results from six samples (left): 10 µL of TOTAL and PAR fractions were loaded on a 2% agarose gel and separated (80 V for 35 min). On the right, there is another gel of sample 2 only, where the prokaryotic rRNAs can be visualized more clearly. Eukaryotic rRNA (18S and 25S) are indicated by black arrowheads and prokaryotic rRNAs (16S and 23S) by grey arrowheads.(D) Example of a Bioanalyzer result of a degraded sample. L: standard ladder. Green line: lower marker present in all lanes. Abbreviations: RIN = RNA integrity number; PAR = polysome-associated mRNA; nt = nucleotides; L = standard ladder. Please click here to view a larger version of this figure.

Since these samples are from symbiotic nodules where eukaryotic and prokaryotic RNAs coexist, the purified RNA is a mix of both species (although the eukaryotic ones are the majority). Hence, it is expected to observe peaks corresponding to 16S and 23S rRNA in the electropherograms (Figure 2B and zoom-in B1 and B2). These "extra" peaks could explain the lower RIN values obtained.

The equipment also calculates sample concentrations considering the standard ladder in lane 1 as a reference. As expected, the TOTAL samples present higher concentration values than the PAR samples. Still, even for these, there is enough RNA to proceed with library preparation and RNA-seq since sample quantity requirements typically recommend at least 1.0 µg.

Autoclavable solutions to be stored at room temperature
2 M Tris-HCl pH 9.0
2 M KCl 
0.5 M EGTA pH 8.0 (adjusted with 10 M NaOH)
1 M MgCl2
20% (v/v) PTE (shake bottle before pipetting the solution)
10% DOC 
20% Detergent mix: 20% (w/v) Brij L23, 20% (v/v) Tritón X-100, Igepal CA 360, 20% (v/v) Tween 20 (dissolve while heating at 60 °C)
Filter-sterilizable solutions to be frozen at -20 °C
0.5 M DTT
0.5 M PMSF
50 mg.mL-1 cycloheximide (CHX) (in EtOH)
50 mg.mL-1 chloranphenicol (CHL) (in EtOH)

Stock solution Volume (µL) for 10 mL PEB Volume (µL) for 2 mL RB
2 M Tris, pH 9.0 1,000 200
2 M KCl 1,000 200
0.5 M EGTA pH 8.0 500 100
1 M MgCl2 356 70
20% (v/v) PTE 500
10% DOC 1,000
20% Detergent mix 500
0.5 M DTT 100 20
0.5 M PMSF 20
50 mg.mL-1 CHX 10 2
50 mg.mL-1 CHL 10 2
H2O 5,004 1,406
2 M sucrose solution (68.5%): 68.5 g of sucrose in water. Keep at room temperature (RT). 
10x salt solution: 0.4 M Tris-HCl pH 8.4, 0.2 M KCl, 0.1 M MgCl2; autoclave for 15 min, freeze at -20 °C. 

Table 1: Buffers and solutions used in this protocol. The volumes given are for six samples. Abbreviations: EGTA = ethylene glycol-bis(2-aminoethylether)-N,N,N´,N´-tetraacetic acid; PTE = polyoxyethylene (10) tridecyl ether; DOC = sodium deoxycholate; DTT = dithiothreitol; PMSF = phenylmethanesulfonyl fluoride.

Sucrose layer (%) Sucrose 2 M (mL) Salt solution 10x (mL) CHX 50 mg.mL-1 (µL) CHL 50 mg.mL-1 (µL) H2O (mL)
12 5.25 3 3 3 21.75
33.5 14.7 3 3 3 12.3

Table 2: Composition of the two sucrose layers (12% and 33.5%). The volumes given are for the preparation of six cushions.

Discussion

Studying gene expression regulation at the translational level is critical to better comprehend different biological processes since the endpoint of cell gene expression is protein abundance13,14. This can be assessed by analyzing the translatome of the tissue or organism of interest for which the polysomal fraction should be purified and its associated mRNAs analyzed3,4,34,35,36.

A method is presented here to purify soybean symbiotic nodule polysomes through sucrose cushions, followed by TOTAL and PAR extraction. Obtaining both RNA fractions is one relevant point of this protocol since RNA-seq and standard pipelines for gene expression could be implemented afterward. Thus, the transcriptome and the translatome of the nodule can be studied.

An alternative method for polysome purification is the translating ribosome affinity purification (TRAP) method, in which the expression of an epitope-tagged version of ribosomal protein L18 allows for the immunoprecipitation of ribosomes37,38. However, this method requires the generation of transgenic plants, which can be challenging for some species such as the soybean. Moreover, the ribosome profiling or Ribo-seq method15,39,40,41, which involves the deep sequencing of ribosome-protected mRNA fragments after polysome purification, is an alternative for studying the translatome with higher resolution than polysome profiling, since the exact number and position of ribosomes on individual mRNAs can be assessed. Nevertheless, this approach is more laborious, requires higher amounts of sample, and is computationally intensive, since small RNA fragments are recovered.

There are several critical experimental aspects to consider, such as the quality of the sample from which the polysomes will be purified, especially if frozen tissue is used, as is the case in this protocol. Intact nodules should be detached from the root and immediately frozen in liquid nitrogen before storage at −80 °C. In our experience, polysomes and their associated mRNAs can be successfully purified from nodules within a few months of storage. Furthermore, the whole protocol must be implemented under conditions that prevent RNA degradation to obtain high-quality TOTAL and PAR, which is critical for downstream applications such as cDNA synthesis and high-throughput sequencing.

A major limitation of the method is the ultracentrifugation step, as ultracentrifuges are not widely available in many laboratories. Also, it is relevant to mention that the pellet obtained after the centrifugation step might contain, besides polysomes, other ribonucleoproteins complexes that are not translationally active. Moreover, one consideration if performing the protocol presented here with another soybean tissue is that it will probably require optimizing the amount of sample, the sample:PEB ratio, and the homogenization procedure.

Considering that the sample used in this protocol is an organ formed due to a symbiotic interaction between a plant root cell and a bacteria, performing a Dual RNA-seq analysis42 (with TOTAL and PAR samples) would be interesting since it would allow examination of the transcriptional and translational responses from both organisms. The method described here could be helpful for this matter if the extraction of the bacterial RNAs is optimized.

Disclosures

The authors have nothing to disclose.

Acknowledgements

This research was funded by CSIC I+D 2020 grant No. 282, FVF 2017 grant No. 210, and PEDECIBA (María Martha Sainz).

Materials

Plant growth and rhizobia inoculation
Orbital shaker Daihan Scientific Model SHO-1D
YEM-medium Amresco J850 (yeast extract) 0122 (mannitol)
Water deficit treatment
KNO3 Merck 221295
Porometer Decagon Device Model SC-1
Scalpel
Preparation of cytosolic extracts
Brij L23 Sigma-Aldrich P1254
Centrifuge Sigma Model 2K15
Chloranphenicol Sigma-Aldrich C0378
Cycloheximide Sigma-Aldrich C7698
DOC Sigma-Aldrich 30970
DTT Sigma-Aldrich D9779
EGTA Sigma-Aldrich E3889
Igepal CA 360 Sigma-Aldrich I8896
KCl Merck 1.04936
MgCl2 Sigma-Aldrich M8266
Plastic tissue grinder Fisher Scientific 12649595
PMSF Sigma-Aldrich P7626
PTE Sigma-Aldrich P2393
Tris Invitrogen 15504-020
Triton X-100 Sigma-Aldrich T8787
Tween 20 Sigma-Aldrich P1379
Weighing dish  Deltalab 1911103
Preparation of sucrose cushions
Sucrose Invitrogen 15503022
SW 40 Ti rotor Beckman-Coulter
Ultracentrifuge Beckman-Coulter Optima L-100K
Ultracentrifuge tubes Beckman-Coulter 344059 13.2 mL tubes
RNA extraction and quality control
Agarose Thermo scientific R0492
Bioanalyzer Agilent Model 2100. Eukaryote total RNA nano assay
Chloroform DI 41191
Ethanol Dorwil UN1170
Isopropanol Mallinckrodt 3032-06
Glycogen Sigma 10814-010
TRIzol LS Ambion 102960028
Miscellaneous
Falcon tubes 15 mL Biologix 10-0152
Filter tips 10 µL BioPointe Scientific 321-4050
Filter tips 1000 µL BioPointe Scientific 361-1050
Filter tips 20 µL BioPointe Scientific 341-4050
Filter tips 200 µL Tarsons 528104
Microcentrifuge tubes 1.5 mL Tarsons 500010-N
Microcentrifuge tubes 2.0 mL Tarsons 500020-N
Sequencing company Macrogen
Sterile 250 mL flask Marienfeld 4110207

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Sainz, M. M., Filippi, C. V., Eastman, G., Sotelo-Silveira, M., Martinez, C. M., Borsani, O., Sotelo-Silveira, J. Polysome Purification from Soybean Symbiotic Nodules. J. Vis. Exp. (185), e64269, doi:10.3791/64269 (2022).

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