shadow-1 and wild-type plants were vegetatively propagated in rectangular pots (15 cm × 11 cm × 5 cm). Plant roots and shoots were cut to 2.5 cm and six groups of two tillers were evenly spread within each pot. Plants were maintained at a 5 cm height in full light for 6 weeks. Individuals selected for shade-stress treatment were placed in a 95% shade environment in the greenhouse, which was created by the use of black polyfiber cloth. Those selected for full-sunlight treatment were left out in the open in the greenhouse. After growing for an additional 2 weeks under either light or 95% shade, leaf tissue was collected from six pots (one biological replicate) for each genotype (wild type or shadow-1) under each treatment (light or shade). A total of three replicates were collected for each genotype under each treatment. Tissue was collected by cutting young leaves directly into a beaker of liquid nitrogen in an effort to preserve mRNA. For shade-treated plants, this was done in a darkroom environment to avoid light contamination.

Total plant RNA was extracted using the RNeasy Plant Mini Kit, including RNase-Free DNase set (Qiagen, Valencia, CA, United States), according to the manufacturer’s protocol. RNA purity and concentration were measured using the NanoDrop 2000 spectrophotometer (Thermo Fisher Scientific, Waltham, MA, United States). To further assess RNA quality, total RNA was analyzed on the Agilent TapeStation 2200 (Agilent Technologies, Santa Clara, CA, United States) using the RNA High Sensitivity assay. Ribosomal Integrity Numbers (RINe) were recorded for each sample. Only samples with RINe values above 7.0 were used for library preparation. Total RNA samples were prepared for mRNA-Sequencing using the Illumina TruSeq Stranded mRNA Sample Preparation kit following the manufacturer’s protocol (Illumina, San Diego, CA, United States). Libraries were validated for length and adapter dimer removal using the Agilent TapeStation 2200 D1000 High Sensitivity assay (Agilent Technologies, Santa Clara, CA, United States) and were then quantified and normalized using the dsDNA High Sensitivity Assay for Qubit 2.0 (Life Technologies, Carlsbad, CA, United States). Libraries were prepared for the Illumina HiSeq 2500 (v.4 chemistry) in High Output mode (2 × 100 bp). A total of 12 libraries were sequenced across two lanes.

Clean reads were obtained by first removing adapter sequences, and then filtering out reads with over 20% low-Q-value (≤20) bases, as well as reads with more than 5% ambiguous “N” bases. The clean reads were then aligned to the perennial ryegrass genome assembled by Byrne et al. (2015) using default parameters in Tophat2 software (Kim et al., 2013). Gene expression levels were calculated as reads per kilobase of transcript per million mapped reads (RPKM). Differentially expressed genes (DEGs) were defined as genes having a false discovery rate (FDR) ≤0.05 and an absolute log₂ fold change value ≥1. To further characterize the function of DEGs, they were mapped to Gene Ontology (GO) classifications using Blast2GO (Conesa and Götz, 2008). Three categories of GO annotations were analyzed: biological process, molecular function, and cellular component. To uncover GA biosynthesis genes and GA response gene of perennial ryegrass, BLASTP was performed against the translated perennial ryegrass reference genome for each gene of interest. The top hits with an E-value <10^-4 were aligned using ClustalX 2.0 (Larkin et al., 2007). A phylogenetic tree was constructed for all selected hits by PHYML version 3.0 using the maximum likelihood method (Guindon et al., 2010) under the JTT evolutionary model. The closest neighbor for each protein was designated as the putative homolog for that protein in perennial ryegrass. A representative phylogenetic tree was provided in the Supplementary File 1.

Three genes: KS, KAO, and GA20ox were analyzed using quantitative real-time PCR (qRT-PCR). New plant material was harvested, and RNA was extracted, as previously described. The iScript^TM cDNA Synthesis Kit (Bio-Rad Laboratories, Richmond, CA, United States) was used to synthesize cDNA, and cDNA products were utilized for qRT-PCR assays using SsoFast^TM EvaGreen^® Supermix (Bio-Rad Laboratories, Richmond, CA, United States) on a CFX96^TM Real-Time PCR detection system (Bio-Rad Laboratories, Richmond, CA, United States). Primer sequences for all genes analyzed are as follows: KS forward: 5′-GGAAACCTGCTAGACTGGAA-3′, KS reverse: 5′-ATTTAGGTACCCGAGGGCTT-3′, KAO forward: 5′-CAGGAAGATGGAGTACCTCT-3′, KAO reverse: 5′-ATGTGCACAGTCCTGTACCA-3′, GA20ox forward: 5′-GACTTCACGCAGAAGCACTA-3′, GA20ox reverse: 5′-GCAGATGCAGAGAAGCAGAA-3′, LpGAPDH forward: 5′-CATCACCATTGTCTCCAACG-3′, LpGAPDH reverse: 5′-AACCTTCAACGATGCCAAAC-3′. The native glyceraldehyde-3-phosphate dehydrogenase (LpGAPDH) gene was used as the internal control (Petersen et al., 2004; Kovi et al., 2016). Data were analyzed using CFX Manager^TM software version 2.0. The expression levels in each sample was normalized using the expression level of LpGAPDH gene in the same sample. Three biological replicates were performed with each type of sample. Means of gene expression levels between shadow-1 and wild type were compared using the two-tailed Student’s t-test with the pooled variance (Steel et al., 1997).

When grown in the greenhouse under full light conditions, shadow-1 plants exhibited dwarfism, categorized by reduced canopy heights compared to wild type (Figure 1A). Following 2 weeks of shade treatment, shadow-1 plants were found to be more tolerant to shade compared to wild type, as evidenced by a significant reduction in leaf elongation and the retention of a healthy, green appearance (Figure 1B). These results are consistent with previously reported analysis of the shadow-1 mutant line (Li et al., 2016).

Following the 2 weeks of shade treatment, leaf tissue samples were harvested from the shadow-1 and wild-type plants, kept under both shade and light conditions, for transcriptome analysis. We used three biological replicates for each genetic background under each treatment. Transcriptome sequencing data were deposited in the NCBI SRA database under the accession number SRP102018. Through sequencing, we generated a total of 657,122,180 raw reads and 633,014,566 clean reads. The average Q20 and Q30 scores for clean reads among all 12 samples were 95.88 and 90.40%, respectively. For these reads, the average GC content was 50.42% (Table 1). We used the perennial ryegrass genome assembled by Byrne et al. (2015) as a reference against which the clean reads from each sample were mapped. We were able to map around 75% of the clean reads for each sample group to the reference genome (Table 2).

We have compared gene expression among the three biological replicates for all four sample types: wild type kept under light, shadow-1 kept under light, wild type treated with shade, and shadow-1 treated with shade. The similarity of expression profiles between the replicates was determined by a Pearson correlation coefficient analysis. We found that the three biological replicates for each sample type were highly correlated (r > 0.96), demonstrating consistency between replicates regarding to DEGs (Figure 2).

When we examined the number of DEGs for each of these four comparisons (Figure 3), we observed that shade treatment caused more changes in gene expression (i.e., more DEGs) than the mutation(s) in shadow-1 plants under either light or shade conditions. These results demonstrate that shade stress has a larger impact on gene expression than the mutation(s).

There were 4,022 DEGs in shade-treated wild-type plants, compared to those which were grown in the light, with 1,392 up-regulated and 2,630 down-regulated. Similarly, there were 4,067 DEGs (1,374 up-regulated and 2,693 down-regulated) in shade-treated shadow-1 plants compared to those kept under light (Figure 3). 2,668 DEGs (820 up-regulated and 1,848 down-regulated) were shared between shade-treated shadow-1 and shade-treated wild-type plants, when each were compared to their light-grown counterparts (Figure 4A). It is likely that many of these genes are not involved in the shade tolerance exhibited by shadow-1 plants, but instead are representative of the general shade response of perennial ryegrass.

There were 2,245 DEGs (1,153 up-regulated and 1,092 down-regulated) uncovered in light-grown shadow-1 plants, compared to wild-type and 2,200 DEGs (1,096 up-regulated and 1,104 down-regulated) uncovered in shade-treated shadow-1 plants, compared to wild type (Figure 3). There were 1,240 DEGs (624 up-regulated and 616 down-regulated) shared by shadow-1 plants under light and shade, when each were compared to wild-type under the same conditions. 1,005 DEGs (529 up-regulated, 476 down-regulated) were found only in light-grown shadow-1 (compared to wild type) and 960 DEGs (472 up-regulated, 488 down-regulated) found only in shade-treated shadow-1 (compared to wild type) (Figure 4B).

We also compared differential gene expression between light-grown shadow-1, shade-treated shadow-1, light-grown wild-type, and shade-treated wild type, in a four-way comparison (Figure 4C). This four-way comparison exposed 329 DEGs that were unique to shadow-1 when compared to wild-type under shade conditions, and 485 DEGs that were unique to shadow-1 if compared to wild type under light conditions. There were also 820 DEGs that were unique to shade-treated wild-type plants (compared to wild type under light), and 889 DEGs that were unique to shade-treated shadow-1 plants (compared to shadow-1 under light). There were 87 DEGs that had differential expression in shadow-1 and wild type under both light and shade.

In order to explore the function of DEGs identified in shadow-1 plants (compared to wild type) under both light and shade conditions, we performed GO enrichment analysis. The enriched GO distributions were similar for shadow-1 plants under light and under shade (compared to wild type under the same conditions), however, there were a few notable differences. We examined some of the genes from the GO groups that showed differences and queried the associated proteins against the NCBI NR protein database. DEGs involved in “biological adhesion” and “receptor activity” for shadow-1 plants kept under light were absent in shadow-1 plants treated with shade (Figure 5). The “biological adhesion” group included a gene that coded for ERECTA, a receptor-like kinase, and was up-regulated (9.85×) in shadow-1 plants compared to wild type under light. The “receptor activity” group included a gene that coded for PhyA, a light receptor, was also up-regulated (7.24×) in shadow-1 plants under light. For another GO group, “extracellular region part,” shadow-1 plants under light had only down-regulated DEGs, while shade-treated shadow-1 plants had both up- and down-regulated DEGs (Figure 5). One gene within this group coded for cytokinin oxygenase, which degrades bioactive cytokinin, and was up-regulated (11.38×) in shadow-1 plants under shade compared to wild type, but was not differentially regulated in shadow-1 under light.

Previously, we showed that the dwarfism and shade-tolerance phenotypes displayed in shadow-1 might be caused by changes in GA concentration (Li et al., 2016). The genes responsible for GA biosynthesis are poorly annotated in perennial ryegrass, but are well characterized in bread wheat (Triticum aestivum), a close relative of perennial ryegrass. To uncover DEGs within the GA biosynthesis pathway, we selected the protein sequences for enzymes catalyzing key steps of GA biosynthesis in bread wheat and aligned them to the translated perennial ryegrass reference genome (Supplementary File 2). As shown in Figure 6, putative GA biosynthesis genes were down-regulated in shadow-1 plants (compared to wild type) under both light and shade conditions. Under light, the GA biosynthesis genes, CPS, KS, KO, and KAO, were down-regulated to 24.4–84.7% of the levels of wild-type plants. Under shade conditions, these genes were also down-regulated to 17.4–61.4% of the wild type plants. The downstream GA biosynthesis splits into two pathways, one for GA₁ and another for GA₄. Both pathways are catalyzed by GA20ox followed by GA3ox, which are responsible for key steps in GA biosynthesis. Expression of GA20ox was reduced in shadow-1 plants kept under light, to 39.0% of the expression in wild type. Under the shade conditions, the expression of GA20ox in shadow-1 plants was reduced to 3.3% when compared to the wild type control. We were unable to uncover putative homologs of GA3ox through annotation.

We next examined one GA response gene, lipid transfer protein 3 (LTP3), which is up-regulated by GA (De Lucas et al., 2008). LTP3 was down-regulated to 41.5% in shadow-1 plants if compared to its expression in wild type under shade conditions (Figure 7). This gene was also down-regulated in shadow-1 plants when comparing to the wild-type under nature light (data not shown).

We verified the accuracy of our transcriptome data by selecting three genes (KS, KAO, and GA20ox) for qRT-PCR analysis, using mRNA extracted from shade-treated wild-type and shadow-1 plants. The results of qRT-PCR analysis showed similar expression patterns to those obtained from our transcriptome analysis (Figure 8). Transcriptome analysis demonstrated that, in shade-treated shadow-1, KS expression was reduced to 17.4% of its expression in wild type, while qRT-PCR showed down-regulation to 14.8% of wild-type expression. Under the same conditions, transcriptome analysis showed that KAO was down-regulated in shadow-1 to 43.3% of its wild-type expression, while qRT-PCR showed down-regulation to 49.7%. For shade-treated shadow-1, GA20ox was down-regulated to 3.3% of its expression in wild type. 3.3% represents a total of only 0.03 mapped reads (RPKM) over millions of sequencing reactions, which is in the barely detectable level. Consistently, we could not detect expression of this gene for these plants with our qRT-PCR analysis. In summary, the expression patterns detected with the transcriptome and qPCR analyses are consistent in general, demonstrating that the transcriptome data from Illumina sequencing analysis are reliable.