A total of 46 samples from 16 different tissues (Table 1) of 10 Dezhou donkeys were collected for RNA sequencing. Eight milk samples (45 ml/sample) from eight other Dezhou donkeys were also collected for quantitative proteomics. Ten donkeys were anesthetized using pentobarbital (100 mg/kg, i.v.) and euthanized by exsanguination. The tissue samples were chopped to small sections and thoroughly washed using DNase-free and RNase-free water. They were placed in liquid nitrogen to freeze and then stored at −20°C. The milk samples were frozen immediately after collection at each milking and stored at −20°C until analysis. A detailed sample information is provided in Supplementary Table 1. The donkeys were utilized in this study in line with protocols of care and use of laboratory animals, following receipt of permission from the Animal Care and Use Committee of Shandong Academy of Agricultural Sciences.

The procedures for RNA sequencing were adopted from a previous study (Wang et al., 2020). In brief, RNA was obtained using TRIzol (Thermo Fisher Scientific, CA, United States) and evaluated with an Agilent 2100 Bioanalyzer (Agilent Technologies, CA, United States). After screening, high-quality RNA was sequenced (RNA integrity number >7.0 and 28S/18S ratio > 1.0). The total RNA was purified using oligo-dT beads. Thereafter, the mRNA strands were fragmented using Fragmentation Buffer (Ambion, Thermo Fisher Scientific, CA, United States). The cDNA libraries were then constructed using the templates. The cDNA was sequenced on the Illumina HiSeq 4000 system for paired-end reads with a read length of 100 bases.

RNA sequencing data was aligned by utilizing HISAT2 software (v2.1.0) (Kim et al., 2019) based on donkey reference sequences (EquAsi1.0, GenBank assembly accession: GCA_016077325.1) as previously described (Wang et al., 2020). StringTie (v2.1.4) was used for transcript assembly and quantification, including fragments per kilobase million (FPKM) and transcripts per million (TPM; Pertea et al., 2015). Novel transcripts and genes were predicted using gffcompare (v0.11.2) (Pertea and Pertea, 2020). The transcripts whose class code was annotated by “u,” length >200 nt, and exon number >1 were retained and subjected to novel gene annotation. DIAMOND, kofamscan, and hmmer were used to annotate novel genes on the basis of five public databases, namely, NCBInr,² SwissProt,³ eggNOG,⁴ Kyoto Encyclopedia of Genes and Genomes (KEGG)⁵, and Pfam,⁶ with >500 bit score, >50% pident, and >1e-20 E-value. Further studies were performed in accordance with the reference genes. In order to compare the donkey mRNA profile with human or other livestock data, we used the classification scheme of Uhlén et al., which was previously developed for human mRNA profiling. The gene and transcript expression levels were estimated based on the average FPKM of each tissue sample (Uhlén et al., 2015). It ratifies the genes into six classes: “not detected” (FPKM <1 in all tissues), “tissue enriched” (fivefold higher FPKM than any other tissue), “group-enriched” (fivefold higher average FPKM in two to seven tissues, relative to the rest of tissues), “expressed in all” (FPKM >1 in all tissues), “tissue-enhanced” (fivefold FPKM higher than the average FPKM of the rest of tissues), and “mixed” (did not match the aforementioned categories).

The principal component analysis (PCA) and hierarchical clustering analysis of individual samples were performed on the TPM for all genes. PCA was generated using the R (v4.0.3) function “prcomp.” In unsupervised hierarchical clustering, the Spearman correlation-based distance for each sample and the average linkage method were used. The clusters were displayed on a heat map developed based on the pairwise correlation coefficients. Heat maps were plotted with the pheatmap R package.

The Cytoscape 3.0 software was adopted to create a network of tissue- and group-enriched genes which were classified on the basis of FPKM (Shannon et al., 2003). The network included the group-enriched nodes with a maximum of five connections and at least three expressed genes. FPKM was used as a measure of gene expression.

Gene Ontology (GO) and pathway enrichment analysis of tissue-enriched and ubiquitously expressed genes, classified on the basis of FPKM, were conducted on ClusterProfiler package (v3.18.0) in R software. P-values were adjusted by false discovery rate (Yu et al., 2012). In accordance with the functional annotation of Uniprot (see text footnote 3), the related protein products of the genes were classified into categories of predicted intracellular proteins, predicted secreted proteins, and genes with isoforms belonging to both categories.

The milk samples in lysis buffer (a mixture of 2 mM EDTA, 1 mM PMSF, 40 mM Tris–HCl, pH 8.5, 4% CHAPS, 2 M thiourea, and 7 M urea) were agitated on ice. Subsequently, the extracted proteins were incubated at 56°C with 10 mM dithiothreitol (final concentration) for 1 h to decrease the number of disulfide bonds. The milk was then alkylated for 1 h in a dark room using 55 mM IAM (final concentration). This mixture was place on chilled acetone (at −20°C), 4 × volume of the milk, overnight to allow precipitation. It was then centrifuged at 30,000 × g under 4°C to form a protein pellet that was reconstituted in 0.5 M TEAB (Applied Biosystems, Milan, Italy) and agitated on ice. The suspension was then centrifuged at 30,000 × g under 4°C, and the protein was quantified with the Bradford assay.

The total protein (100 μg) from each milk sample was heated at 37°C for 16 h using Trypsin Gold (Promega, Madison, WI, United States). The digestion was done at a ratio of 1:20, i.e., trypsin to protein. Thereafter, the protein digests were dried in vacuum through centrifugation. The peptide cocktails were suspended in 0.5 M TEAB and then treated with 8-plex iTRAQ reagent (Applied Biosystems), following the protocols of the manufacturer.

The labeled peptide cocktail was first fractioned on the LC-20AB HPLC Pump system (Shimadzu, Kyoto, Japan) and thereafter suspended in 4 ml buffer A mixture (25 mM NaH₂PO₄ in 25% ACN, pH 2.7). The peptides were loaded onto a 4.6 × 250-mm Ultremex SCX column mixed with 5-μm particles (Phenomenex). Elution was performed at 1 ml/min for 10 min using buffer A. The second elusion was performed for 27 min using 5–60% buffer B (25 mM NaH₂PO₄ and 1 M KCl in 25% ACN, pH 2.7) before the final elusion for 1 min using 60–100% buffer B. The peptides were added into 100% buffer B and allowed to incubate for 1 min before equilibrating using buffer A for 10 min prior to the next injection. The absorbance of the peptide cocktail was measured regularly at 214 nm to monitor the progress of elution. Samples were also obtained at 1 min each. Finally, 20 fractions of the peptides were pooled together before desalting using Strata X C18 column (Phenomenex). The peptides were then dried in vacuum.

The peptide extracts were resuspended in buffer A (a mixture of 2% CAN and 0.1% FA) before centrifugation at 20,000 × g for 10 min. Thereafter, 10 μl of the supernatant was added onto an LC-20AD nano HPLC (Shimadzu, Kyoto, Japan) and eluted. Loading of samples was performed at the rate of 8 μl/min for 4 min before running at 300 nl/min for 44 min. The concentration of B (a mixture of 98% CAN and 0.1% FA) started from 2 to 35% and thereafter at 80% for 2 min, at 80% B for 4 min, and finally at 5% for 1 min.

Nanoelectrospray ionization of the peptides was performed before the tandem mass spectrometry (MS). The latter process was performed in Q EXACTIVE HPLC (Thermo Fisher Scientific, San Jose, CA, United States). An Orbitrap operating at a resolution of 70,000 was employed to identify unbroken peptides. Ion fragments were detected using an Orbitrap at a resolution of 17,500. The voltage for electrospray was 1.6 kV. The automatic gain control target for full MS and MS2 were 3e6 and 1e5, respectively. The m/z scan range of the MS scans was 350–2,000 Da and 100–1,800 m/z for MS2 scans.

Raw data generated from the Orbitrap were converted into MGF files by using Proteome Discoverer 1.2. The Mascot search engine, v2.3.02 (Matrix Science, London, United Kingdom), was adopted to identify the proteins on the NCBInr and SwissProt databases. The iTRAQ-identified proteins were matched to the GO,⁷ COG, and KEGG databases for protein functional annotation. A mass tolerance of 20 ppm was used for identifying intact peptides, whereas 0.05 Da was used for fragmented ions. Up to one missed cleavage in the trypsin digests was allowed. Only peptides correctly selected at 95% confidence interval based on Mascot probability were chosen to decrease the probability of false identification of peptides. Moreover, each confident protein identification involved at least one unique peptide. An intensity-based absolute quantification (iBAQ) algorithm was used to estimate the absolute protein abundance ranking (Schwanhäusser et al., 2011).

FASTA of bovine milk (Tacoma et al., 2016), sheep milk (Ha et al., 2015), swine milk (Ogawa et al., 2014), and human milk (Gao et al., 2012) was downloaded from UniprotKB⁸ to compare the protein ingredient of human milk with the milk of other mammals. Then, BLASTP was used to match the protein sequences of bovine milk, sheep milk, and swine milk (query argument) to human milk (subject argument). The alignment of BLASTP was based on an E-value of 1E-5 and identity ≥30%.

Sixteen histologically healthy tissue specimens representing major donkey organs were analyzed by RNA sequencing (Table 1). Overall, 22,303 protein-coding genes and 68,480 transcripts were assembled from the mapped reads. A total of 6,290 novel genes and 24,514 novel transcripts were predicted, of which 1,365 were annotated by comparison with NR (621 novel genes), SwissProt (535 novel genes), eggNOG (922 novel genes), KEGG (151 novel genes), and Pfam (674 novel genes; intensity-based absolute quantification). Simultaneously, 16,013 protein-coding genes and 21,983 transcripts were successfully mapped to the reference genome. Further studies based on the reference genes were performed.

The global expression profiles were investigated using PCA and hierarchical clustering on the basis of the correlation between 46 samples from 16 organs and tissues (Figures 1A,B). TPM was used as a measure of gene expression. The PCA revealed the testis and the brain as outliers, as also confirmed by hierarchical clustering analysis. Moreover, the hierarchical clustering analysis results uncovered the connectivity between the samples from the two striated muscle samples (cardiac and skeletal muscles), the hematopoietic organ spleen and blood, and the skin and chestnut.

A list of genes in each tissue is shown in Figure 1C. Gene classification was achieved on the basis of mRNA level (FPKM). The number of genes detected in the blood and epididymis averaged 10,035 and 12,987, respectively. The average FPKM for different tissues and organs ranged from 1 to >10,000 (Figure 1D).

All coding genes were classified as previously reported (Uhlén et al., 2015) to explore the proteins with a tissue-specific expression profile (Figure 2A and Supplementary Table 3). The average FPKM was used as a measure of gene expression. The largest group of genes (∼42%, n = 6,778/16,013) was expressed in all tissues. However, ∼47% (n = 7,559/16,013) of all genes were over-expressed in at least one tissue (“tissue-enriched,” “group-enriched,” or “tissue-enhanced”). The tissue-enriched genes constituted ∼16% (n = 2,601/16,013) of all genes, with ∼3% (n = 503/16,013) highly tissue-enriched with at least 50-fold over-expression of mRNA as exemplified by the breast enriched with α-lactalbumin (LALBA), the lung enriched with surfactant protein, and the brain enriched with myelin-associated oligodendrocyte basic protein. The group-enriched and tissue-enhanced genes comprised ∼10% (n = 1,627/16,013) and ∼21% (n = 3,331/16,013) of all genes, respectively. Furthermore, 3% of all genes (n = 502/16,013) were not detected in any tissues analyzed in this study.

Transcriptomic and network analyses (Figures 2B,C) revealed that only 1.0% (on average) of all genes showed a tissue-enriched profile. The brain (4.1%, n = 653/16,013) and the testis (6.5%, n = 1,048/16,013) were the notable exceptions, which displayed a substantially higher percentage of tissue-enriched genes. The transcriptomic analysis also allowed the determination of the fraction of elevated transcripts in each tissue. For the majority of tissues, ∼27% of the transcripts were encoded by tissue-elevated genes, except the muscle and the liver where the elevated genes encoded 58.0 and 58.4% of the transcripts, respectively. The network plot showed the number of tissue-enriched genes for each tissue and group-enriched genes shared with another tissue. The skin and chestnut shared many group-enriched genes as expected due to the similar cells consisting the tissues. As a hematopoietic organ, the spleen shared 76 group-enriched genes with blood. A notable detail is that the brain also shared several group-enriched genes with the gonads.

The functional categories and subcellular localizations of genes specifically expressed in certain tissues accurately reflected the long-standing function of tissues—for instance, many of the tissue-enriched genes of the testis were intracellular, while most tissue-enriched genes were secreted in the breast and the liver (Figure 3A). GO analysis revealed that the majority of testis-specific genes participated in spermatid development, differentiation, and motility (Figure 3B and Supplementary Table 4). The function of the testis to produce sperm was compatible with the subcellular localization of its tissue-enriched genes. By contrast, LYZ and LALBA encoding for secreted proteins LYSC1 and LALBA were specifically and highly expressed in the breast. Furthermore, the most abundant tissue-specific proteins for the liver were plasma proteins, e.g., albumin, haptoglobin, and many proteins that belonged to the cytochrome P450 superfamily of enzymes.

A functional KEGG pathway analysis for the tissue-enriched genes of 16 tissues is summarized in Figure 3C and Supplementary Table 5, and the results were consistent with the function of each tissue—for example, the heart-enriched genes encoded proteins that are involved in cardiac muscle contraction, the skin-enriched genes encoded proteins that are associated with lipid metabolism, and the brain-enriched genes were involved in functions related to signaling pathways and synapse. The brain-, heart-, and muscle-enriched genes were also observed to be involved in adrenergic signaling in cardiomyocytes and the calcium signaling pathway. The brain- and stomach-enriched genes participated in gastric acid secretion.

The transcriptomic analysis revealed that close to 7,000 genes (Supplementary Table 3) were expressed in all analyzed tissues. According to the result of the pathway analysis, these housekeeping gene regulates the structure and function of cellular organelles, such as transcription, translation, protein processing, proteolysis, transport, signal transduction, and energy metabolism (Figure 3D and Supplementary Table 6).

In view of the high lysozyme content in donkey milk, LYZ and LALBA genes and their protein products were subsequently studied in depth. Seven c-type (chicken or conventional type; i.e., LYZ, LALBA, LYZL1, LYZL4, LYZL6, SPACA5, and SPACA3) and two g-type (goose type; i.e., LYG1 and LYG2) lysozyme genes were detected to be expressed in different donkey tissues (Figure 4A). LYZL1, LYZL4, LYZL6, SPACA5, and SPACA3 were highly expressed in the reproductive system, including the testis and the epididymis; LYG1 and LYG2 were highly expressed in the skin, and LYZ and LALBA were breast-enriched genes. Simultaneously, 265 proteins in donkey milk were quantified via the iBAQ method. The results showed that β-lactoglobulin-1, β-casein, LALBA, LYSC1, and κ-casein were the top five proteins with the highest content in donkey milk (Supplementary Table 7). According to protein annotation, LYZ, which encodes the LYSC1 protein, is an orthologous gene in donkey and horse. LYSC1 is a unique lysozyme protein to Equus. The IBQA analysis showed a high LYSC1 content in donkey milk. Furthermore, no other lysozyme proteins were found in donkey milk. The lysozyme concentration was 1.0 g/L in donkey milk, 0.79 g/L in mare milk, and 0.5 g/L in human milk, whereas it showed a trace amount in bovine, sheep, and swine milk (Table 2). Given that those intact LYZ genes that predict potentially functional LYSC1 were found in only a few species (e.g., donkey and horse), the high expression of LYZ in donkey breast may lead to a high lysozyme content in donkey milk.

Moreover, a total of 401 non-redundant proteins in donkey milk were identified by the iTRAQ method (Table 3 and Supplementary Figure 1), of which 381 were annotated by comparison with GO (235 proteins), COG (182 proteins), and KEGG (373 proteins) databases (Supplementary Table 8 and Supplementary Figures 2–4). In particular, the KEGG pathway enrichment analysis revealed that proteins were mainly enriched in immune and inflammatory response-related pathways, such as complement and coagulation cascades, lysosome, and phagosome. After a BLASTP search was conducted, 285 proteins in donkey milk, representing 71% of total self-proteins, were found to overlap with human milk proteins. Moreover, the number of overlapping proteins in bovine, sheep, and swine milk was 292 (representing 31% of total self-proteins), 210 (32%), and 33 (18%), respectively, (Figure 4B).