PLoS ONEplosplosonePLoS ONE1932-6203Public Library of ScienceSan Francisco, USAPONE-D-13-4504010.1371/journal.pone.0088216Research ArticleBiologyComputational biologyMicroarraysGeneticsMolecular geneticsGene regulationGene expressionGenetics of diseaseHuman geneticsMedicineAnatomy and physiologyRespiratory systemRespiratory physiologyPulmonologyRespiratory infectionsCiliary Genes Are Down-Regulated in Bronchial Tissue of Primary Ciliary Dyskinesia PatientsDown-Regulation of Ciliary Genes in PCDGeremekMaciej123*ZiętkiewiczEwa4BruinenbergMarcel2FrankeLude2PogorzelskiAndrzej5WijmengaCisca23WittMichał14International Institute of Molecular and Cell Biology, Warsaw, PolandGenetics Department, University Medical Centre Groningen and University of Groningen, Groningen, the NetherlandsComplex Genetics Group, Department of Biomedical Genetics, University Medical Center Utrecht, Utrecht, the NetherlandsDepartment of Molecular and Clinical Genetics, Institute of Human Genetics, Poznan, PolandInstitute of Tuberculosis and Lung Diseases, Rabka, PolandRoySudiptoEditorInstitute of Molecular and Cell Biology, Singapore* E-mail: macgerem@gmail.com
The authors have declared that no competing interests exist.
Conceived and designed the experiments: MG CW MW. Performed the experiments: MG MB. Analyzed the data: MG LF EZ. Contributed reagents/materials/analysis tools: AP. Wrote the paper: MG EZ.
201462201492e8821641120135120142014Geremek et alThis is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Primary ciliary dyskinesia (PCD) is a rare, genetically heterogeneous disease characterized by recurrent respiratory tract infections, sinusitis, bronchiectasis and male infertility. The pulmonary phenotype in PCD is caused by the impaired motility of cilia in the respiratory epithelium, due to ultrastructural defects of these organelles. We hypothesized that defects of multi-protein ciliary complexes should be reflected by gene expression changes in the respiratory epithelium. We have previously found that large group of genes functionally related to cilia share highly correlated expression pattern in PCD bronchial tissue. Here we performed an explorative analysis of differential gene expression in the bronchial tissue from six PCD patients and nine non-PCD controls, using Illumina HumanRef-12 Whole Genome BeadChips. We observed 1323 genes with at least 2-fold difference in the mean expression level between the two groups (t-test p-value <0.05). Annotation analysis showed that the genes down-regulated in PCD biopsies (602) were significantly enriched for terms related to cilia, whereas the up-regulated genes (721) were significantly enriched for terms related to cell cycle and mitosis. We assembled a list of human genes predicted to encode ciliary proteins, components of outer dynein arms, inner dynein arms, radial spokes, and intraflagellar transport proteins. A significant down-regulation of the expression of genes from all the four groups was observed in PCD, compared to non-PCD biopsies. Our data suggest that a coordinated down-regulation of the ciliome genes plays an important role in the molecular pathomechanism of PCD.
This work was covered in part by the grant NN401 095537 from the Ministry of Science and Higher Education, Poland and by the grant BESTCILIA [305404, Better Experimental Screening and Treatment for Primary Ciliary Dyskinesia (7FP, HEALTH.2012.2.4.4-2)]. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.Introduction
Cilia are small cellular projectiles, extending from the cell surface, with which they share the cell membrane. The ciliary axoneme is built on a scaffold of nine peripheral microtubule doublets, associated with many multi-protein complexes, including outer and inner dynein arms (ODA and IDA), nexin links and radial spokes. Cilia act either as sensors (primary cilia) or propel fluid over the epithelia of various organs (motile cilia) [1]; their dysfunction is the underlying cause of many systemic diseases.
Primary ciliary dyskinesia (PCD) is a rare genetic disease characterized by recurrent respiratory tract infections, bronchiectasis and infertility. Pulmonary symptoms occur because of the lack of an efficient mucociliary clearance, caused by the kinetic dysfunction of motile cilia in the respiratory epithelium. Male infertility is caused by the dysmotility of flagella in spermatozoids. Situs inversus, a mirror reversal of body organ positioning, is present in approximately half of the PCD patients because of the immotility of primary cilia of the embryonic node [2], [3]. In rare cases, PCD symptoms are a part of syndromic diseases, e.g. X-linked retinitis pigmentosa [4], [5] and oral-facial-digital type I syndrome [6]. The diagnosis of PCD is based on the clinical criteria, the delayed saccharin test [7], and low levels of nasal nitric oxide [8]. These symptoms are supported by the imaging studies of the respiratory cilia. Tissue specimens obtained through bronchoscopy are evaluated in the light microscope for ciliary beating and with the electron microscope for defects of the ciliary ultrastructure. Among a wide spectrum of various ultrastructural ciliary lesions documented in PCD patients [9], the lack of ODA and/or IDA is the most frequently observed defect.
Genetically, PCD is a largely autosomal recessive trait with extensive heterogeneity. To date, nineteen genes have been found to be mutated in PCD: DNAH5[10], DNAH11[11], DNAI1[12], DNAI2[13], RSPH9[14], RSPH4A[14], TXNDC3[15], KTU/PF13[16], LRRC50[17], [18], CCDC39[19], CCDC40[20], CCDC103[21], HEATR2[22], LRRC6[23], DNAL1[24], DNAAF3[25], HYDIN[26], CCDC114[27],CCDC164[28], CCDC65[29], c21orf59[30], SPAG1[31], ZMYND10[32], RSPH1[33], ARMC4[34], and DYX1C1/DNAAF4[35]; additional genes are involved in syndromic forms of PCD: RPGR[4], [5] and OFD1[6]. Products of most of the PCD-related genes have conserved orthologs in Chlamydomonas reinhardtii and have a well-defined ultrastructural localization in the axoneme. However, the large complexity of the cilium, which is composed of hundreds of proteins, renders studying the ciliary function a difficult task. In effect, the genetic basis of PCD in about half of patients remains unknown.
Previously, in search for a better understanding of the molecular basis of functional defects of cilia in PCD, we have performed the whole-genome expression profiling in bronchial biopsies from six PCD patients [36]. Clustering analysis revealed a large group of genes with highly correlated expression pattern in PCD biopsies, but not in controls; based on the series of in silico analyses, we have indicated over 200 new genes potentially involved in the biology of human cilia. In the present study, we further explored the gene expression profiling data to characterize patterns of differential gene expression in bronchial tissue from PCD patients and non-PCD controls. We report that the significant proportion of genes that are down-regulated in PCD encode specific elements of the cilium, suggesting that a coordinated down-regulation of the ciliome genes plays an important role in the molecular pathomechanism of PCD.
Materials and MethodsEthics statement
The Institutional Review Board (IRB) of the Medical University of Poznań approved use of bronchial biopsy specimens of patients and controls for genetic studies on PCD. Specimens were collected during routine hospital procedures. Written informed consent was obtained from all subjects.
Bronchial biopsies and subjects
Material for this study, obtained from six unrelated PCD patients and nine unrelated control individuals, has been described in detail in Geremek et al. [36]. Briefly, clinical evaluation of the PCD patients was performed at the Institute of Tuberculosis and Lung Diseases in Rabka, Poland, by the experienced physician (AP). The primary bronchopulmonary symptoms in the patients were: sinusitis, nasal polyps, bronchiectasis, and recurrent infections of the upper respiratory tract. PCD status was also indicated by the positive results of routine diagnostic tests: the delayed saccharine test and lack of the ciliary motility in light microscopy imaging. In four patients (#1, 2, 3, 4), PCD diagnosis was confirmed by the low level of NO (25–188 ppb), measured in the nasal cavity (chemiluminescence analyzer, the threshold value of 200 ppb) [8] (Table S1). Three of these patients (#1, 3, 4) had ODA/IDA defect. One patient (#6) for whom no NO data were available had IDA defect and another one (#5) in whom NO level was in the normal range had ODA/IDA defect. Two of the patients (#5, 6) had situs inversus. The mutational status was known for one patient (patient #4), who was a compound heterozygote for two mutations in DNAH5. Non-PCD controls were individuals referred to the Institute of Tuberculosis and Lung Diseases in Rabka for various reasons unrelated to PCD; they presented no symptoms of acute pulmonary disease, no bronchoscopic signs of the disturbance of mucociliary transport, and had normal ciliary beating in the light microscopy.
Biopsies were obtained during a diagnostic bronchoscopy, using the same protocol in PCD and non-PCD individuals. Specimens were stored in RNAlater buffer and used for RNA isolation.
Gene expression analysis
The quality and concentration of RNA were determined using the 2100 Bioanalyzer (Agilent, Amstelveen, The Netherlands) with the Agilent RNA 6000 Nano Kit. Anti-sense RNA was synthesized, amplified and purified using the Ambion Illumina TotalPrep Amplification Kit (Ambion, USA) according to the manufacturer's protocol. Complementary RNA was hybridized to Illumina HumanRef-12 Whole Genome BeadChips and scanned on the Illumina BeadArray Reader. Data was handled through the Illumina BeadStudio Gene Expression module v3.2. The expression data has been submitted to GEO under accession number GSE25186.
Data-analysis
Initial steps of data preprocessing, quantile normalization, background subtraction and quality control were performed using the BeadStudio software. The data were exported to GeneSpring 9. Expression values with a threshold value below 5 were raised to 5, and the data were scaled by a base 2 logarithm.
Ensembl Biomart module was used to obtain Ensemble gene IDs of the differentially expressed genes that were subject to annotation enrichment analysis and the Ciliome database (www.ciliome.com) [37] search. Fold-change analysis for all the probes was performed using GeneSpring 9 software. Genes that had at least 2-fold expression change (with the t-test p-value <0.05) in PCD patients as compared to the controls were subjected to gene annotation enrichment analysis using DAVID (Database for Annotation, Visualization, and Integrated Discovery) [38]. DAVID applies a modified Fisher exact test, to establish if the proportion of genes falling into an annotation category differs for a particular group of genes and the background group of genes; the p-values were corrected for multiple testing using the FDR method. The resulting annotation terms were then clustered into functional groups.
PubMed was used as references for known ciliary genes encoding components of radial spokes and intraflagellar transport proteins. Outer and inner dynein arms genes were taken from Pazour et al [39]. The R package was used for statistical calculations.
The log2-transformed mean expression values for the probes representing protein components of the specific ultrastructural ciliary elements were compared in the patients and controls, and the Wilcoxon Mann-Whitney test was used to obtain p-values for individual comparisons. In case of genes represented by multiple probes, mean values were used for calculations. The unweighted Z-method of combining probabilities from independent tests was used to assess if the distribution of p-values deviated from normal [40]. The Z-transform test converts one-tailed p-values from each of the independent tests into standard normal deviates; the sum of these standard normal deviates, divided by the square root of the number of tests, has a standard normal distribution if the common null hypothesis is true.
ResultsWhole genome analysis (fold change and gene enrichment)
We identified 1323 genes (1396 probes), which displayed at least 2-fold difference in the expression level in PCD compared to non-PCD bronchial tissue (t-test p-value <0.05); 721of these genes (755 probes) were over-expressed, whereas 602 genes (641 probes) showed a reduced expression in PCD (Table S2).
To investigate the biological meaning of these differentially expressed genes, we performed annotation enrichment analysis, separately for the up-regulated and down-regulated genes, using DAVID software [38]. Annotations of the genes with the reduced expression in PCD patients were significantly enriched for terms related to microtubules, motility, cilia, and dyneins (Table 1). In the group of up-regulated genes, the highest scoring cluster was related to cell cycle and mitosis (Table 2). To investigate how many of the down- and up-regulated genes were functionally linked to cilia, the two groups (genes from Table S2) were used to query the Ciliome database [37]. This search revealed that 19% of the down-regulated and 11% of the up-regulated genes were related to cilia. Under a theoretical assumption that approximately 10% of the human genes are related to cilia (the Ciliome database contains 2024 entries), the proportion of ciliary genes found in the down-regulated group was significantly higher than in the whole set of human genes (binominal p-value 1.69e-08), while the list of up-regulated genes was not significantly enriched for genes related to cilia (p-value 0.26).
10.1371/journal.pone.0088216.t001
Gene annotation analysis of the genes down-regulated in PCD (fold change >2.0, and p<0.05).
Annotation Cluster 1
Enrichment Score: 7.25
Ontology term
Count#
P_Value
FDR*
cilium
23
3.6E-14
1.1E-11
axoneme
15
6.2E-14
9.9E-12
microtubule
30
9.6E-13
1.0E-10
microtubule cytoskeleton
42
1.9E-12
1.5E-10
dynein complex
13
2.6E-12
1.6E-10
cell projection part
26
3.2E-11
1.3E-9
dynein heavy chain, N-terminal region 2
9
5.7E-10
4.1E-7
microtubule motor activity
14
9.2E-9
5.2E-6
microtubule associated complex
15
3.3E-8
8.0E-7
ciliary or flagellar motility
7
2.3E-7
3.8E-4
cytoskeleton
59
2.9E-7
6.6E-6
PIRSF002308:dynein heavy chain, ciliary
6
5.6E-7
8.0E-5
cilium biogenesis/degradation
7
2.4E-6
1.2E-4
ATPase, AAA+ type, core
12
3.5E-4
6.1E-2
non-membrane-bounded organelle
75
3.9E-3
6.3E-2
cell projection organization
16
1.2E-2
9.5E-1
cell motility
10
2.1E-1
1.0E0
Annotation Cluster 2
Enrichment Score: 2.92
Ontology term
Count#
P_Value
FDR*
nucleotide phosphate-binding region:ATP
39
4.6E-4
1.1E-1
purine nucleotide binding
63
6.1E-4
1.1E-1
ribonucleotide binding
60
9.9E-4
1.1E-1
nucleotide binding
69
1.9E-3
1.1E-1
adenyl ribonucleotide binding
50
2.0E-3
1.0E-1
Annotation Cluster 3
Enrichment Score: 2.82
Ontology term
Count#
P_Value
FDR*
cilium morphogenesis
7
5.9E-5
2.5E-2
cilium assembly
6
2.7E-4
8.9E-2
cell projection organization
16
1.2E-2
9.5E-1
cell part morphogenesis
12
2.1E-2
9.4E-1
cell projection assembly
6
3.2E-2
9.8E-1
Count is a non-exclusive number of genes in each annotation category.
False discovery rate.
10.1371/journal.pone.0088216.t002
Gene annotation analysis of the genes up-regulated in PCD (fold change >2 and p<0.05).
Annotation Cluster 1
Enrichment Score: 8.84
Ontology term
Count#
P_Value
FDR*
cell cycle
47
7.6E-12
1.4E-8
M phase
30
8.5E-12
7.7E-9
mitotic cell cycle
29
7.0E-10
2.5E-7
cell division
22
6.0E-9
1.0E-6
nuclear division
21
1.0E-8
3.0E-6
organelle fission
21
2.0E-8
4.5E-6
Annotation Cluster 2
Enrichment Score: 5.81
Ontology term
Count#
P_Value
FDR*
intracellular non-membrane-bounded organelle
84
3.2E-8
9.6E-6
cytoskeleton
40
3.6E-3
5.3E-2
Annotation Cluster 3
Enrichment Score: 4.93
Ontology term
Count#
P_Value
FDR*
translational elongation
14
7.2E-8
1.3E-5
structural constituent of ribosome
16
4.5E-7
2.1E-4
large ribosomal subunit
10
3.2E-6
4.9E-4
ribonucleoprotein
18
6.8E-6
4.7E-4
translation
20
2.5E-5
3.0E-3
ribonucleoprotein complex
23
1.9E-4
5.6E-3
Annotation Cluster 4
Enrichment Score: 3.86
Ontology term
Count#
P_Value
FDR*
regulation of cell cycle
25
2.8E-8
5.7E-6
regulation of organelle organization
14
3.2E-4
3.1E-2
regulation of mitosis
6
4.5E-3
2.2E-1
Annotation Cluster 5
Enrichment Score: 3.04
Ontology term
Count#
P_Value
FDR*
condensed chromosome
12
2.3E-5
1.0E-3
chromosome
23
3.6E-5
1.3E-3
kinetochore
7
2.8E-3
4.5E-2
centromere
4
2.7E-2
3.9E-1
Count is non-exclusive number of genes in each annotation category.
False discovery rate.
Known ciliary genes
To search for the evidence of differential expression of the genes related to specific elements of the axonemal ultrastructure, we assembled a list of human proteins represented on the microarray and predicted to be a part of the known ultrastructural ciliary components (ODA, IDA, radial spokes, intraflagellar transport-related proteins). We used the data from Pazour et al. [39], who applied phylogenetic analysis to assign human heavy dynein chains to ultrastructural components of outer and dyneins arms of flagella, and from Hom et al. [41], who compiled data on the nomenclature of dyneins. The assignment of the remaining genes was based on the PubMed search.
The resulting list of 37 human genes encoding proteins predicted to be a part of known ciliary components included: 8 ODA genes, 10 IDA genes, 8 radial spoke genes and 11 intraflagellar transport genes (Table 3). The log 2-transformed mean expression levels in PCD and non-PCD bronchial tissues, the fold change, the log2 of the fold change and the corresponding Wilcoxon Mann-Whitney test p-values are presented in Table 3. All the genes had a lower expression in PCD than in controls. Statistically significant evidence of the down-regulation in PCD was also observed when the combined p-values were calculated, using an unweighted Z-method [33], in four subgroups of the genes encoding ciliary components: ODA (p = 3.5e-08), IDA (p = 3.19e-12), radial spokes (p = 1.06e-4) and intraflagellar transport proteins (p = 1.27e-07), respectively (Table 3).
10.1371/journal.pone.0088216.t003
Differential expression of the genes encoding outer dynein arms, inner dynein arms, radial spokes and intraflagellar transport proteins in the group of PCD cases compared to the non-PCD controls.
Gene#
PCD Log2 of the expression
Non-PCD Log2 of the expression
Regulation
Log2 of the fold change nonPCD/PCD
Fold change nonPCD/PCD
Wilcoxon Mann-Whitney one tail p-value
Z-method combined p-value
Inner dynein arms
3.188885e-12
DNAH1
7.099971713
8.823093021
Down
1.72312131
3.301499231
0.002397602
DNAH10#
2.845467386
2.930532774
Down
0.08506539
1.060735818
0.297612503
DNAH12L
2.984792693
4.691691968
Down
1.70689927
3.264584241
0.005496876
DNAH2
8.605120088
10.73227718
Down
2.12715709
4.368557834
0.001398601
DNAH3
5.76933297
8.094913833
Down
2.32558086
5.012675559
0.005605302
DNAH7
6.514024915
8.269907386
Down
1.75588247
3.377328402
0.003796204
DNHD2
8.860690672
10.45193877
Down
1.59124809
3.01309903
0.017982018
DNHL1#
2.704540406
3.102569317
Down
0.39802891
1.317706357
0.069468652
WDR63
6.410269672
8.011632917
Down
1.60136324
3.034298967
0.017982018
WDR78#
4.278425094
5.226285631
Down
0.94786054
1.92900989
0.024775225
Outer dynein arms
3.524812e-08
DNAH11
3.002922837
5.663426945
Down
2.66050411
6.322539346
0.002598476
DNAH5
2.840433314
5.349519237
Down
2.50908592
5.692592858
0.010311612
DNAH9#
4.195042679
4.979603695
Down
0.78456102
1.722568101
0.008791209
DNAI1
8.674843985
9.844952993
Down
1.17010901
2.250286995
0.033166833
DNAI2
7.177192762
8.6898654
Down
1.51267264
2.853381481
0.002397602
DNAL1#
5.239162724
5.900496355
Down
0.66133363
1.58154393
0.163836164
TCTE1
3.213232157
4.82357751
Down
1.61034535
3.053249212
0.007662144
TCTE3
2.361725905
2.586822518
Down
0.22509661
1.168855518
0.617456403
Radial spokes
0.0001061203
RSPH3
7.413315798
7.836831773
Down
0.42351598
1.341192183
0.227972028
RSHL3 (RSPH4A)#
9.513876417
10.3676621
Down
0.85378569
1.807236971
0.136063936
NME5 (RSPH23)
9.938877607
10.88896095
Down
0.95008335
1.931984273
0.264335664
RSPH1
10.4069913
11.50297723
Down
1.09598593
2.137591135
0.072327672
C6ORF206 (RSPH9)
8.57029857
9.296022759
Down
0.72572419
1.653730552
0.163836164
RSPH10B#
4.839311246
5.755622796
Down
0.91631155
1.887284017
0.005994006
PPIL6 (RSPH12)
6.766706564
8.011535825
Down
1.24482926
2.369905052
0.111888112
DNAJB13
4.103136217
5.749770835
Down
1.64663462
3.131024115
0.033166833
Intraflagellar transport complex
1.275819e-07
DYNC2H1
6.048332879
8.057745569
Down
2.00941269
4.026182839
0.002397602
DYNC2LI1#
5.614105936
5.886374416
Down
0.27226848
1.20770532
0.264335664
IFT122#
4.919297327
5.396632088
Down
0.47733476
1.39216939
0.008791209
IFT140
6.501863507
7.674088316
Down
1.17222481
2.253589598
0.017982018
IFT172
8.232366019
9.177805846
Down
0.94543983
1.925775902
0.017982018
IFT52#
6.3875103
6.531748043
Down
0.14423774
1.105146586
0.303496503
IFT57
8.12299147
9.303622084
Down
1.18063061
2.266758367
0.033166833
IFT74
7.712753509
8.095831669
Down
0.38307816
1.304121386
0.227972028
IFT80#
2.430337143
2.764181897
Down
0.33384475
1.260367755
0.100406593
IFT81#
3.80548032
4.32006191
Down
0.51458159
1.428579763
0.194205794
IFT88#
4.97817553
5.909540297
Down
0.93136477
1.907079214
0.033166833
# In case of genes represented by multiple probes, mean values were used for calculations
The results were not dependent on individual PCD patients. Removing of each of the PCD subject did not significantly change the result of gene annotation analysis. Evidence of the down-regulation in four subgroups of the genes encoding ciliary components remained also significant.
Discussion
A combination of the fold change with the significance measured by an uncorrected t-test (which takes into consideration the variance between the samples), has been shown to be a reliable and reproducible measure of differential expression [42].The gene expression profiling using the whole-genome Illumina panel, performed in bronchial biopsies from six PCD patients and nine non-PCD controls, revealed 1396 probes (representing 1323 genes) with at least 2 fold expression level difference between the PCD and non-PCD groups (t-test p-value <0.05). Functional annotation of the differentially expressed genes revealed that those down-regulated in PCD were related to microtubules, motility and cilia, and the up-regulated ones to the cell cycle and mitosis, i.e. to the processes that are related to microtubules by mitotic spindle and centrioles.
To further characterize the expression changes in PCD, we analyzed expression levels of a number of cilia-related genes represented on the chip. We assembled the list of 37 human genes representing: three subgroups, related to the ultrastructural components of motile cilia (outer dynein arms, inner dynein arms, and radial spokes), plus one functional subgroup (intraflagellar transport proteins). In all these subgroups, the reduced expression in bronchial biopsies from PCD patients was observed. The largest number of probes exhibiting significantly decreased expression was observed in the group of genes encoding components of inner and outer dynein arms.
Of the twenty-six genes known to be mutated in PCD, CCDC39, CCDC164 and SPAG1 were not represented on the array and TXNDC3 was not stably expressed. Of the remaining twenty-two stably expressed genes (Table 4), ten were significantly down-regulated (>2-fold change and p<0.05). The majority of the down-regulated PCD genes encoded components of cilia ultrastructure: ODA (DNAH11, DNAH5, DNAI1, DNAI2, DNAL1, CCDC114); central pair appendix (HYDIN). The remaining down-regulated PCD genes encoded cytoplasmic proteins required for the assembling of dynein arms (LRCC50 alias DNAAF1, ZMYND10). In twelve of the PCD genes the expression level did not significantly differ between PCD and non-PCD biopsies; five of these genes (KTU alias DNAAF2, CCDC103, DYX1C1, c21orf59 and C19ORF52 alias DNNAAF3) encoded cytoplasmic assembly proteins, two (CCDC40 and CCDC65) encoded N-DRC (nexin-denein regulatory complex) proteins, one (HEATR2) encoded protein of an unknown location and three encoded radial spokes proteins (RSPH4A, RSPH1 and RSPH9), one (ARMC4) encoded ODA docking component; only the expression of DNAAF3 and CCDC40 was slightly higher in PCD than in healthy controls. ODF1 associated with the syndromic form of PCD, was expressed at the significantly lower lever in PCD patients. DYX1C1, LRCC6, RPGR, RSPH1 had the fold change >2 but the p-values were between 0.05 and 0.1.
10.1371/journal.pone.0088216.t004
Differential expression of the genes mutated in PCD and two genes mutated in syndromic disorders associated with PCD symptoms (RPGR and ODF1).
Gene#
Probe ID
PCD Log2 of the expression
Non-PCD Log2 of the expression
Regulation
Log2 of the fold change nonPCD/PCD
Fold change nonPCD/PCD
T-test p-value
ARMC4
4200274
8,327165
9,390315
down
1,06315
2,089488
0,130237
C19ORF52 (DNAAF3)
6290253
7.118648
6.746589
up
−0.372059
0.77267895
0.132469
C21ORF59*
7040162
10,05058
10,54353
down
0,492947
1,407317
0,212658
C6ORF206 (RSPH9)
840433
8.570299
9.296023
down
0.72572
1.653725749
0.135019
CCDC103
6770463
7.065492
7.691135
down
0.62564
1.542895124
0.240855
CCDC114
7210482
6.548517
8.35885
down
1.81033
3.507225031
0.017073
CCDC40*
4150072
2.886536
2.4908
up
−0.395737
0.76010098
0.150259
CCDC65
2370228
7,4877
8,417493
down
0,929793
1,905002
0,151083
DNAH11*
7330360
3.002923
5.663427
down
2.6605
6.322521334
0.004405
DNAH5
2350554
2.840433
5.349519
down
2.50909
5.692608957
0.003368
DNAI1
2810300
8.674844
9.844953
down
1.17011
2.250288539
0.040018
DNAI2
5960685
7.177193
8.689865
down
1.51267
2.85337626
0.006119
DNAL1*
6100682
3.770269
5.508203
down
1.73793
3.335562329
0.007245
DYX1C1*
3140523
4,361447
5,485308
down
1,123861
2,179294
0,071072
HEATR2*
5290037
8.210407
8.386503
down
0.1761
1.129825525
0.494105
HYDIN*
7550360
6.950931
9.07216
down
2.12123
4.350647105
0.000905
KTU (DNAAF2)
2490408
6.58843
6.791816
down
0.20339
1.151400704
0.579292
LRRC50 (DNAAF1)
5550035
8.577057
10.22783
down
1.65077
3.140011842
0.010513
LRRC6
2350477
6.796389
7.90332
down
1.10693
2.153868244
0.08437
ODF1
3120427
2.669272
3.925799
down
1.25653
2.38920393
0.046691
RPGR*
2750386
2.726082
3.783812
down
1.05773
2.081653578
0.065558
RSHL3 (RSPH4A)*
2630519
9.918507
10.80253
down
0.88402
1.845510569
0.187161
RSPH1
6020451
10,40699
11,50298
down
1,095986
2,137591
0,105587
ZMYND10
4540066
8,938617
10,15335
down
1,214728
2,320971
0,012449
In case of genes represented by multiple probes, the most significant probe is shown.
TXNDC3 was not stably expressed, CCDC39, CCDC164 and SPAG1 were not represented on the array.
Given the lack of linear relation between RNA and protein, direct conclusions about a possible correlation between the RNA level and ultrastructural ciliary defects cannot be made. Large multi-protein complexes of the dynein arms are pre-assembled in the cytoplasm, before their intraflagellar transport to the ciliary axonemes. Immunohistochemical staining of the ciliated epithelium from PCD patients with identified mutations has shown that a defect/absence of one of the ciliary proteins may impair the delivery or assembly of other, non-mutated members of the axonemal substructures [43]. This relationship has been shown e.g. for mutated DNAH5 or DNAI1 and DNAH9 [43], mutated KTU and components of ODA/IDA [16], mutated CCDC40 or CCDC39 and components of IDA [19], [20], mutated LRRC6 and components of ODA/IDA [23]. Our data suggest that this impairment of the ciliary ultrastructure assembly may in fact originate at the transcription level; we hypothesize that a regulatory system may exist, which – in the presence of a mutated ciliary gene – down-regulates the expression of at least part of the ciliary genome. Such a regulation would play an important role in the molecular pathomechanism of PCD. During ciliogenesis the expression of ciliary genes is regulated by common transcription factors. The FOXJ1 transcription factor and RFX (regulatory factor X) family of transcription factors have been shown to regulate the expression of many cilia related genes. We have found FOXJ1 (FC = 2,086838) and RFX2 (FC = 2,412601) among the down-regulated genes indicating that the putative regulatory event acts upstream of these two transcription factors[44].
In our study, the strongest evidence of a significant down-regulation of the cilia-related genes in PCD bronchial biopsies concerned the genes predicted to encode elements of the inner and outer dynein arms and to a lesser extent, elements of radial spokes and proteins involved in ODA assembly or in the intraflagellar transport. The small study group provides only the proof of the concept and further studies are warranted. For example, to estimate the specificity of a putative regulatory system it will be important to repeat similar analyses using groups of patients carrying mutations in the same gene. In our small group of patients, only one of the patients had a known mutational status (two complementary heterozygous mutations in DNAH5). DNAH5 is the strongest contributor to the genetic background of PCD, but one cannot exclude the possibility that there were mutations in other genes among the patients we examined. One may envision that the homogeneous group of patients with the mutations in the specific genes would cause different groups of the ciliary genes to undergo down-regulation.
Apart from the contribution to the understanding of the mechanisms of ciliary assembly, such studies may contribute to finding further candidate genes in PCD. To date, a number of candidate disease genes in several genomic regions reported to be linked to PCD remain to be identified; the failure of many linkage studies may be ascribed to the noise in linkage data, and difficulties in the functional prioritization of the candidate genes. In this context, observation of a down-regulation of the particular gene's expression in PCD might provide clues for selecting candidate genes from the linkage peaks.
Supporting Information
Electron microscopy, NO measurements and situs status in the PCD patients studied.
(DOCX)
Differentially expressed genes (fold change >2 and p<0.05).
(DOC)
The cooperation of all the Polish families who participated in this study was invaluable. We thank Jackie Senior for editing the manuscript and Ewa Rutkiewicz for laboratory assistance. We thank the staff of the Genomics Facility, UMCG, for scientific and technical work. MG was supported by the International PhD Program of the University of Utrecht.
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