Abstract
Bovine spongiform encephalopathy (BSE) is a fatal, transmissible, neurodegenerative disease of cattle. To date, the disease process is still poorly understood. In this study, brain tissue samples from animals naturally infected with BSE were analysed to identify differentially regulated genes using Affymetrix GeneChip Bovine Genome Arrays. A total of 230 genes were shown to be differentially regulated and many of these genes encode proteins involved in immune response, apoptosis, cell adhesion, stress response and transcription. Seventeen genes are associated with the endoplasmic reticulum (ER) and 10 of these 17 genes are involved in stress related responses including ER chaperones, Grp94 and Grp170. Western blotting analysis showed that another ER chaperone, Grp78, was up-regulated in BSE. Up-regulation of these three chaperones strongly suggests the presence of ER stress and the activation of the unfolded protein response (UPR) in BSE. The occurrence of ER stress was also supported by changes in gene expression for cytosolic proteins, such as the chaperone pair of Hsp70 and DnaJ. Many genes associated with the ubiquitin-proteasome pathway and the autophagy-lysosome system were differentially regulated, indicating that both pathways might be activated in response to ER stress. A model is presented to explain the mechanisms of prion neurotoxicity using these ER stress related responses. Clustering analysis showed that the differently regulated genes found from the naturally infected BSE cases could be used to predict the infectious status of the samples experimentally infected with BSE from the previous study and vice versa. Proof-of-principle gene expression biomarkers were found to represent BSE using 10 genes with 94% sensitivity and 87% specificity.
Introduction
Transmissible spongiform encephalopathies (TSEs), also termed prion diseases, are fatal, neurodegenerative diseases including Creutzfeldt-Jakob disease (CJD) in humans, scrapie in goats and sheep and bovine spongiform encephalopathy (BSE) in cattle [1], [2], [3], [4]. The infectious agent of these diseases is thought to be an abnormally folded isoform (PrPSc) of the cellular prion protein (PrPC) and it is further thought that the accumulation of the misfolded prion protein leads to disease [1]. PrPSc is characterized by a high β-sheet content and resistance to protease treatment. In addition to the accumulation of PrPSc, the pathological features of prion diseases in the brain of affected subjects include neuronal cell loss and vacuolation. Prion diseases have long incubation periods prior to the onset of clinical signs.
BSE was first discovered in 1986 [5] and became a major epidemic in the UK, peaking in 1992; to date more than 185,000 cases have been recorded. It is thought to be caused by contaminated meat and bone meal, a dietary supplement for cattle [6]. The BSE strain has also most probably crossed the species barrier to humans and has produced variant CJD [7]. The mean incubation period of BSE in cattle is estimated at about 5 years [3]. The clinical signs are: difficulties in locomotion and behavioural changes. The neuropathology of BSE is characterized by the lesions mainly found in the brain stem where vacuolar changes are found in neurons and the neuropil [5]. However, apoptosis plays a very limited role in neuronal loss in BSE [8].
In recent years atypical bovine spongiform encephalopathy has been identified [9], [10]. In these cases the distribution of PrPSc in the animal differs from that of BSE; there is less PrPSc accumulation in the brain stem and the biochemical signature of PrPSc is different.
The pathogenesis of BSE is still poorly understood. In a previous gene expression study using brain tissue samples from cattle experimentally infected with BSE, we have demonstrated that the largest number of differentially regulated genes is detected at 21 months post inoculation, suggesting that there are many pathogenic processes in the animal brain even prior to the detection of infectivity in the CNS of these orally dosed cattle [11]. Moreover, a set of differentially regulated genes could be used to predict the infectious status of preclinical samples.
To further understand the pathogenesis of BSE and to explore the possibility of using gene expression profiles as biomarkers, we analysed brainstem RNA samples from confirmed naturally infected cases of BSE (field cases) in cattle and from healthy controls.
Results
Identification of differentially regulated genes in the BSE field case samples
The expression of genes in the brain of naturally infected BSE samples was compared with negative controls. In order to identify differentially regulated genes in BSE, the following stringent conditions were set with two filters: 2 fold change and one-way ANOVA with the p value being 0.05. 409 probe sets (a technical term that describes a transcript on the microarray) were identified as differentially regulated between the BSE infected (n = 14) and negative (n = 12) samples. After removal of duplications, 230 genes were identified and these genes are listed in Table 1 and the unannotated probe sets are listed in Table S1.
Table 1. Relative levels of differentially expressed genes of BSE.
| Gene ID | Gene Nams | Fold | p-value | |
| change | ||||
| Cell adhesion | Bt.23129.3.S1 | similar to Laminin gamma-1 chain precursor (Laminin B2 chain) | 2.70 | 0.0209 |
| Bt.2573.1.S1 | CD9 antigen (p24) | 3.61 | 0.0164 | |
| Bt.4817.2.S1 | claudin 11 | 5.38 | 0.019 | |
| Bt.8382.2.S1 | ras homolog gene family, member B | 2.14 | 0.0119 | |
| Bt.11224.1.S1 | similar to 85 kDa lysosomal sialoglycoprotein | 2.83 | 0.0266 | |
| Bt.15742.1.S2 | CD47 molecule | 2.04 | 0.0316 | |
| Bt.18378.1.S1 | similar to KIAA1014 protein | 2.29 | 0.0401 | |
| Bt.4653.1.S2 | platelet/endothelial cell adhesion molecule | 3.57 | 0.0399 | |
| Apoptosis | Bt.5250.1.S1 | milk fat globule-EGF factor 8 protein | 2.58 | 0.035 |
| Bt.222.1.S1 | crystallin, alpha B | 2.07 | 0.0469 | |
| Bt.13130.1.S1 | tumor necrosis factor receptor superfamily, member 5 | −2.33 | 0.0469 | |
| Bt.16079.1.S1 | reticulon 3 * | 2.10 | 0.041 | |
| Bt.21430.1.S1 | similar to Synovial apoptosis inhibitor 1, synoviolin | 5.18 | 0.0237 | |
| Bt.16916.1.S1 | TGF-beta inducible early growth response protein 2 | 2.24 | 0.028 | |
| Bt.23228.1.S1 | Similar to Fas apoptotic inhibitory molecule 2 | 2.74 | 0.041 | |
| Bt.2408.1.S1 | chemokine (C-C motif) ligand 2 | −3.07 | 0.0428 | |
| Bt.8220.1.A1 | similar to transforming acidic coiled coil 1 | 2.21 | 0.0242 | |
| Immune | Bt.9504.1.A1 | putative MIP1-beta protein | −4.55 | 0.0239 |
| responses | Bt.24900.1.S1 | similar to T-cell immunomodulatory protein | 2.2 | 0.0141 |
| Bt.29761.1.S1 | T-cell receptor beta chain variable segment | −4.69 | 0.0172 | |
| Bt.26847.1.S1 | linker for activation of T cells | −2.75 | 0.0423 | |
| Bt.4060.1.S1 | T-cell differentiation protein Mal | 2.87 | 0.0109 | |
| Bt.4175.2.S1 | similar to minor histocompatibility antigen 13 | 3.69 | 0.0467 | |
| Bt.3791.1.S1 | basigin | 2.11 | 0.0401 | |
| cell cycle & | Bt.22534.1.S1 | similar to peripheral myelin protein 22 | 2.69 | 0.0171 |
| growth | Bt.11059.1.S1 | Putative tumor suppressor LUCA15) (G15 protein | 2.85 | 0.0084 |
| Bt.2214.1.S1 | similar to prostacyclin-stimulating factor; PGI2-stimulating factor; PSF | 2.09 | 0.0164 | |
| Bt.2220.2.A1 | selenoprotein P, plasma, 1 | 2.45 | 0.0171 | |
| Bt.4750.1.S1 | transketolase | 2.04 | 0.0219 | |
| Bt.29157.1.A1 | growth arrest-specific 2 like 1 | −2.58 | 0.0438 | |
| Bt.29718.2.A1 | growth hormone receptor | −4.46 | 0.0129 | |
| Bt.51.1.S1 | cyclin-dependent kinase 5 | 3.60 | 0.049 | |
| Extracellular | Bt.23250.6.A1 | alpha-2-HS-glycoprotein | 5.68 | 0.0249 |
| Bt.28584.1.S1 | canopy 3 homolog | 3.97 | 0.0288 | |
| Bt.5313.1.S1 | matrix metallopeptidase 2 | 2.90 | 0.0427 | |
| cell proliferation | Bt.4529.1.S1 | farnesyltransferase, CAAX box, beta | 2.65 | 0.0119 |
| & differentiation | Bt.5224.1.S1 | dihydropyrimidinase-like 2 | 2.52 | 0.0172 |
| Bt.435.1.S1 | TIMP metallopeptidase inhibitor 2 | 2.91 | 0.0069 | |
| Bt.1537.1.S1 | N-myc downstream regulated gene 1 | 2.18 | 0.0261 | |
| Transport | Bt.10135.1.A1 | similar to solute carrier family 35, member A5 | 2.76 | 0.0138 |
| Bt.13535.1.A1 | similar to hippocampus abundant transcript-like 1 | 2.42 | 0.0289 | |
| Bt.15466.1.A1 | unc-50 homolog | 2.78 | 0.0475 | |
| Bt.26510.1.S1 | Proteolipid protein | 2.08 | 0.0264 | |
| Bt.23637.1.S1 | adaptor-related protein complex 3, mu 1 subunit | 2.08 | 0.0375 | |
| Bt.21740.1.S1 | transmembrane emp24-like trafficking protein 10 | 2.14 | 0.0499 | |
| Bt.13583.1.A1 | similar to ATP-binding cassette transporter G1 | 2.14 | 0.0484 | |
| Bt.903.1.S1 | similar to choline transporter-like protein 1, splice | 2.94 | 0.0052 | |
| Bt.21168.1.A1 | synaptophysin-like 1 | 2.02 | 0.0201 | |
| Bt.16001.1.S1 | similar to sterol 27-hydroxylase | 2.16 | 0.0272 | |
| Bt.3418.1.S1 | mitochondrial carrier homolog 1 | 2.15 | 0.0447 | |
| Bt.15804.1.S1 | similar to chloride channel protein 3 | 2.22 | 0.0175 | |
| Bt.20007.1.S1 | ATP-binding cassette, sub-family C (CFTR/MRP), member 5 | 2.12 | 0.0471 | |
| Bt.21424.1.A1 | similar to receptor Pit2 | 2.14 | 0.041 | |
| Bt.22735.1.S1 | similar to synaptotagmin-like 2 | 2.27 | 0.022 | |
| Bt.2331.1.A1 | similar to receptor activity-modifying protein 1 | 2.15 | 0.0145 | |
| Bt.23500.1.S1 | secretory carrier membrane protein 4 | 2.23 | 0.024 | |
| Bt.23518.2.S1 | similar to tetracycline transporter-like protein | 2.07 | 0.0122 | |
| Bt.23606.1.S1 | inositol 1,4,5-triphosphate receptor, type 1 | 3.53 | 0.0455 | |
| Bt.269.1.S1 | ATPase, Ca++ transporting, type 2C, member 1 | 2.03 | 0.0312 | |
| Bt.26994.1.A1 | potassium voltage-gated channel, Shal-related subfamily, member 2 | −3.54 | 0.0298 | |
| Bt.27129.1.S1 | similar to solute carrier family 39 (zinc transporter), member 9 | 2.04 | 0.0335 | |
| Bt.3414.3.A1 | HIV-1 Rev binding protein | 2.12 | 0.0312 | |
| Bt.4335.1.S1 | similar to protoporphyrinogen oxidase | 3.57 | 0.0204 | |
| Bt.4430.1.S2 | similar to vacuolar H+-ATPase subunit | 2.09 | 0.0349 | |
| Bt.4977.1.S2 | insulin-like growth factor 2 receptor | 2.07 | 0.0399 | |
| Bt.5000.1.S1 | coatomer protein complex, subunit gamma 2 | 2.00 | 0.0416 | |
| Bt.5293.1.S1 | ATPase, H+ transporting, lysosomal 16 kDa, V0 subunit c | 2.5 | 0.0428 | |
| Bt.5293.2.A1 | proteolipid protein 1 | 2.4 | 0.0141 | |
| Bt.5336.1.A1 | transferrin | 3.22 | 0.0084 | |
| Bt.6096.1.S1 | similar to Conserved oligomeric Golgi complex component 2 | 5.41 | 0.0171 | |
| Bt.7134.1.S2 | glycolipid transfer protein | 2.38 | 0.0143 | |
| Bt.8822.1.A1 | similar to inward rectifier potassium channel Kir1.2 | 2.76 | 0.0203 | |
| Bt.9853.1.S1 | similar to Solute carrier family 25 member 14 | 4.35 | 0.0324 | |
| Bt.26889.1.S1 | solute carrier family 33 (acetyl-CoA transporter), member 1 | 2.11 | 0.039 | |
| Bt.4646.1.S1 | solute carrier family 2 (facilitated glucose transporter), member 1 | 2.35 | 0.0171 | |
| Bt.3208.1.S1 | DDHD domain containing 2 | 2.0 | 0.0306 | |
| Bt.10202.1.S1 | reticulon 4 | 2.53 | 0.024 | |
| Bt.5073.1.S1 | transmembrane emp24 protein transport domain containing 4 | 3.91 | 0.0499 | |
| Proteolysis | Bt.20121.1.S1 | cathepsin D | 2.81 | 0.0164 |
| Bt.20030.1.S1 | calpain 7 | 2.25 | 0.0315 | |
| Bt.12302.1.S1 | plasminogen activator, tissue | 2.59 | 0.0203 | |
| Bt.23840.1.S1 | similar to subtilisin-like proprotein convertase 4 | 4.35 | 0.0175 | |
| Bt.289.1.S1 | pregnancy-associated glycoprotein 16 | −4.53 | 0.0475 | |
| Bt.3888.1.S1 | protein phosphatase methylesterase 1 | 3.77 | 0.0427 | |
| Bt.393.1.S1 | cathepsin B | 2.18 | 0.0401 | |
| Bt.5462.1.S2 | similar to dynein, cytoplasmic, heavy polypeptide 1 | 2.1 | 0.0349 | |
| Bt.1613.1.S1 | protease, serine, 11 | 2.6 | 0.0373 | |
| Bt.7240.1.S1 | leucine aminopeptidase 3 | 2.65 | 0.0344 | |
| Bt.27314.1.A1 | Similar to Cgi67 serine protease | 2.17 | 0.0427 | |
| Signal transduction | Bt.5546.1.S1 | guanine nucleotide binding protein (G protein), alpha inhibiting activity polypeptide 1 | 2.02 | 0.0267 |
| Bt.9163.1.A1 | purinergic receptor P2Y, G-protein coupled, 10 | −2.28 | 0.0249 | |
| Bt.21275.1.S1 | splA/ryanodine receptor domain and SOCS box containing 3 | 4.90 | 0.0351 | |
| Bt.27421.1.S1 | rho/rac guanine nucleotide exchange factor (GEF) 2 | 2.78 | 0.0303 | |
| Bt.2235.1.S2 | GDP dissociation inhibitor 1 | 2.07 | 0.0416 | |
| Bt.24236.1.S1 | deleted in liver cancer 1 | 2.43 | 0.0226 | |
| Bt.12694.1.S1 | similar to Tumor necrosis factor receptor superfamily member 21 precursor (TNFR-related death receptor-6) (Death receptor 6) | 3.53 | 0.0242 | |
| Bt.21758.1.A1 | Down syndrome critical region gene 1-like 1 | 2.77 | 0.0194 | |
| Bt.20511.1.S1 | similar to Ral guanine nucleotide dissociation stimulator A | 2.15 | 0.0175 | |
| Bt.26841.1.A1 | GTPase activating Rap/RanGAP domain-like 3 | 2.02 | 0.0069 | |
| Bt.2846.1.A1 | similar to ras homolog gene family, member U | 2.7 | 0.0175 | |
| Ubiquitin cycle | Bt.2211.1.S1 | ubiquitin-activating enzyme E1 (A1S9T and BN75 temperature sensitivity complementing) | 2.19 | 0.0421 |
| Bt.23266.1.S1 | WW domain containing E3 ubiquitin protein ligase 2 | 2.26 | 0.0312 | |
| Bt.5408.1.A1 | ubiquitin carboxyl-terminal esterase L1 (ubiquitin thiolesterase) | 3.19 | 0.0226 | |
| Bt.20361.1.S1 | F-box and leucine-rich repeat protein 20 | 2.28 | 0.0356 | |
| Bt.13185.1 | ubiquitin-like modifier activating enzyme 2 | 2.0 | 0.0209 | |
| Bt.3753.1.S1 | similar to KIAA0614 protein | 2.43 | 0.0477 | |
| Bt.7651.1.S1 | ankyrin repeat and SOCS box-containing 11 | 2.61 | 0.0476 | |
| Lipid metabolic process | Bt.4040.1.S1 | platelet-activating factor acetylhydrolase, isoform Ib, gamma subunit 29 kDa | 2.18 | 0.0119 |
| Bt.1229.1.S1 | apolipoprotein A-I | 3.72 | 0.0138 | |
| Bt.5467.1.S1 | prosaposin | 4.07 | 0.0242 | |
| Bt.6334.1.A1 | degenerative spermatocyte homolog 1, lipid desaturase | 2.63 | 0.0203 | |
| Bt.12718.1.A1 | Similar to Apolipoprotein D precursor (Apo-D) | 3.75 | 0.0119 | |
| Bt.19709.1.S1 | LAG1 homolog, ceramide synthase 2 | 2.71 | 0.016 | |
| Bt.2342.1.S1 | similar to phosphatidate cytidylyltransferase 2 | 2.02 | 0.023 | |
| Bt.18340.1.A1 | similar to choline/ethanolaminephosphotransferase 1 | 3.06 | 0.007 | |
| protein folding | Bt.23161.2.A1 | heat shock 70 kDa protein 1A | 4.61 | 0.0275 |
| Bt.6149.1.S1 | glucose-regulated protein 170 | 2.3 | 0.0203 | |
| Bt.8686.1.S1 | glucose-regulated protein 94 | 2.33 | 0.0311 | |
| Bt.514.1.S1 | DnaJ (Hsp40) homolog, subfamily C, member 6 | 2.34 | 0.0242 | |
| Kinase | Bt.1020.1.S1 | similar to CDC-like kinase 1 | 2.35 | 0.0483 |
| Bt.9070.2.S1 | centaurin, alpha 1 | 2.54 | 0.0209 | |
| Bt.16200.1.A1 | WNK lysine deficient protein kinase 2 | −2.8 | 0.0319 | |
| Bt.13980.1.A1 | Creatine kinase, mitochondrial 2 | 2.08 | 0.0237 | |
| Bt.19517.1.S1 | v-erb-b2 erythroblastic leukemia viral oncogene homolog 3 (avian) | 2.43 | 0.0242 | |
| Bt.21540.1.S1 | fibroblast growth factor receptor 2 | 2.7 | 0.0119 | |
| Bt.22053.1.S1 | nuclear receptor binding protein 2 | 2.25 | 0.0271 | |
| Bt.22649.1.A1 | focal adhesion kinase | −3.82 | 0.0481 | |
| Bt.4413.1.S1 | diacylglycerol kinase, eta | 3.05 | 0.0324 | |
| Bt.729.1.S1 | similar to TYRO3 protein tyrosine kinase | 2.47 | 0.0119 | |
| Bt.9194.1.S1 | similar to microtubule associated serine/threonine kinase 2 | 2.42 | 0.0247 | |
| Transcription or | Bt.21228.1.A1 | PAX interacting (with transcription-activation domain) protein 1 | 4.44 | 0.0323 |
| Translation | Bt.1078.2.S1 | Nuclear factor of activated T-cells, cytoplasmic | 2.74 | 0.044 |
| Bt.20542.1.S1 | Transcription factor jun-B | −2.17 | 0.0261 | |
| Bt.20473.1.A1 | similar to KIAA0833 protein | 2.35 | 0.0175 | |
| Bt.2418.1.S1 | Similar to KIAA0934 protein | 3.04 | 0.0324 | |
| Bt.17848.1.S1 | similar to transcriptional repressor BSR/RACK7/PRKCBP1 | 2.54 | 0.0126 | |
| Bt.19585.1.S1 | similar to TFIIH basal transcription factor complex p62 subunit | 2.23 | 0.0276 | |
| Bt.21110.1.S1 | similar to neuroblastoma-amplified protein | 3.94 | 0.0375 | |
| Bt.4804.2.A1 | Cyclin-dependent kinase inhibitor 1C (p57, Kip2) | 2.33 | 0.0455 | |
| Metabolism | Bt.21917.1.S1 | pyridoxal (pyridoxine, vitamin B6) phosphatase | 2.76 | 0.0069 |
| Bt.3162.1.S1 | procollagen-proline, 2-oxoglutarate 4-dioxygenase | 2.21 | 0.0119 | |
| Bt.23559.1.S1 | similar to thiamin pyrophosphokinase 1 | 2.06 | 0.0119 | |
| Bt.15925.1.S1 | epoxide hydrolase 2, cytoplasmic | 2.51 | 0.0349 | |
| Bt.27130.1.S1 | Saccharopine dehydrogenase | 2.04 | 0.0212 | |
| Bt.13710.1.S1 | phosphatidylglycerophosphate synthase 1 | 3.17 | 0.049 | |
| Bt.21376.1.S1 | STT3, subunit of the oligosaccharyltransferase complex, homolog | 2.24 | 0.0446 | |
| Bt.20890.1.S1 | amylase, alpha 2B (pancreatic) | 3.38 | 0.0141 | |
| Bt.24210.1.S1 | acyl-CoA synthetase long-chain family member 1 | 2.22 | 0.0319 | |
| Bt.1237.1.S1 | A kinase (PRKA) anchor protein (yotiao) 9 | 2.11 | 0.0286 | |
| Bt.25525.1.A1 | Similar to Ectonucleotide pyrophosphatase/phosphodiesterase 2 | 2.72 | 0.0186 | |
| Bt.1330.1.S1 | aldo-keto reductase family 1, member B1 (aldose reductase) | 2.87 | 0.0172 | |
| Bt.22011.1.S1 | O-linked N-acetylglucosamine (GlcNAc) transferase | 2.12 | 0.0416 | |
| Bt.5002.1.S1 | glycerol-3-phosphate dehydrogenase 1 | 2.15 | 0.0447 | |
| Bt.7951.1.S1 | sphingomyelin phosphodiesterase 1, acid lysosomal | 2.32 | 0.016 | |
| Bt.9126.1.S1 | similar to sterol-C5-desaturase-like | 2.67 | 0.0441 | |
| Bt.5517.1.S1 | 2′,3′-cyclic nucleotide 3′ phosphodiesterase | 3.12 | 0.0387 | |
| Bt.24519.1.S1 | similar to holocarboxylase synthetase | 2.25 | 0.0266 | |
| Bt.25539.1.A1 | similar to Heparan sulfate glucosamine 3-O-sulfotransferase 5 | 2.26 | 0.0209 | |
| Bt.3284.2.A1 | Asparagine-linked glycosylation 3 homolog | −2.02 | 0.0069 | |
| DNA or RNA | Bt.22982.1.A1 | reticulon 1 | 2.56 | 0.0335 |
| binding | Bt.10510.1.S1 | H2A histone family, member X | 2.49 | 0.0167 |
| Bt.26546.1.S1 | MUS81 endonuclease homolog | 3.76 | 0.0288 | |
| Bt.22310.1.S1 | ariadne homolog 2 | 2.28 | 0.0141 | |
| Bt.22356.1.S1 | AT rich interactive domain 1A | 2.60 | 0.0482 | |
| Bt.20959.1.S1 | polymerase (DNA directed), alpha 2 (70 kD subunit) | −3.65 | 0.0373 | |
| Bt.2594.1.S1 | splicing factor, arginine/serine-rich 2 | 2.13 | 0.049 | |
| Bt.15534.1.S1 | tubulin, alpha 1 | 2.26 | 0.0355 | |
| Bt.11182.2.S1 | GC-rich sequence DNA-binding factor homolog | 2.16 | 0.0052 | |
| Bt.27445.1.A1 | similar to ELAV-like protein 3 | 2.25 | 0.0476 | |
| Bt.8206.1.S1 | splicing factor, arginine/serine-rich 7, 35 kDa | 2.05 | 0.0264 | |
| Bt.13659.1.S1 | similar to pre-mRNA processing 8 protein | 2.0 | 0.0475 | |
| Bt.13529.1.S1 | similar to splicing factor 3b, subunit 1 | 2.1 | 0.0474 | |
| Bt.15754.1.S1 | similar to nucleolysin TIAR | 2.16 | 0.0141 | |
| Bt.18270.2.S1 | similar to GW182 autoantigen | 2.54 | 0.0209 | |
| Bt.19937.1.S1 | similar to carboxypeptidase D | 2.18 | 0.0203 | |
| Bt.20304.2.S1 | similar to proliferation potential-related protein | 2.53 | 0.0447 | |
| Bt.21440.1.S1 | similar to DEAD box polypeptide 17 isoform p82 | 2.1 | 0.0261 | |
| Bt.28464.2.S1 | splicing factor, arginine/serine-rich 4 | 2.92 | 0.0242 | |
| Protein binding | Bt.10723.1.S1 | similar to RING finger protein 13 | 2.92 | 0.0129 |
| Bt.11149.1.S1 | vimentin | 2.38 | 0.0141 | |
| Bt.20175.1.S1 | HLA-B associated transcript 5 | 5.0 | 0.0175 | |
| Bt.26104.1.A1 | WAS protein family, member 1 | 2.17 | 0.0272 | |
| Bt.13983.1.A1 | metadherin | 2.01 | 0.0399 | |
| Bt.22603.1.S1 | leucine rich repeat transmembrane neuronal 1 | −2.56 | 0.036 | |
| Bt.12039.1.S1 | protein arginine methyltransferase 2 | 2.70 | 0.04 | |
| Bt.18229.1.A1 | similar to partner and localizer of BRCA2 | 4.22 | 0.0469 | |
| Bt.12825.1.S1 | similar to Actin, aortic smooth muscle (Alpha-actin-2) | 4.54 | 0.049 | |
| Bt.1690.1.S1 | similar to goliath protein | 2.05 | 0.0318 | |
| Bt.1766.1.S1 | actin related protein 2/3 complex subunit 1A | 2.16 | 0.0467 | |
| Bt.29710.1.A1 | tight junction protein 3 | −2.71 | 0.04 | |
| Membrane | Bt.10179.1.S1 | liprin beta1 | 3.77 | 0.0375 |
| protein | Bt.1076.1.S1 | arylsulfatase A | 2.20 | 0.0203 |
| Bt.5447.1.S1 | natriuretic peptide receptor B/guanylate cyclase B | 2.07 | 0.0105 | |
| Bt.13265.1.A1 | similar to plasmolipin | 2.77 | 0.0165 | |
| Bt.23589.2.S1 | signal sequence receptor, alpha | 2.19 | 0.0418 | |
| Bt.22858.1.S1 | uroplakin 3B | −2.3 | 0.0335 | |
| Bt.5636.1.S1 | similar to Exocyst complex component 1 | 2.07 | 0.0307 | |
| Bt.13940.1.S1 | similar to CDC91 cell division cycle 91-like 1 | 2.39 | 0.0206 | |
| Bt.14205.1.S1 | LMBR1 domain containing 1 | 2.57 | 0.0119 | |
| Bt.3625.1.S1 | transmembrane protein 85 | 2.16 | 0.0414 | |
| Bt.15878.1.S1 | similar to LanC-like protein 1 (40 kDa erythrocyte membrane protein) | 3.24 | 0.0097 | |
| Bt.20013.1.S1 | similar to ELOVL family member 7, elongation of long chain fatty acids | 2.5 | 0.0138 | |
| Bt.20219.1.S1 | similar to phosphatidyl inositol glycan class T | 2.37 | 0.0385 | |
| Bt.6405.1.S1 | myelin basic protein | 4.85 | 0.0303 | |
| Bt.22251.1.A1 | similar to chemokine-like factor super family 4 | 3.51 | 0.0385 | |
| Bt.23354.1.S1 | similar to epoxide hydrolase 1 | 2.63 | 0.0139 | |
| Bt.5333.1.S1 | cysteine-rich with EGF-like domains 1 | 2.31 | 0.0399 | |
| Bt.2606.1.S1 | lysosomal-associated membrane protein 2 | 3.17 | 0.0151 | |
| Bt.3904.1.S1 | thioredoxin-related transmembrane protein 2 | 2.99 | 0.0399 | |
| Bt.488.1.S2 | phospholipase A2 receptor 1, 180 kDa | 2.26 | 0.0309 | |
| Bt.24941.1.S1 | abhydrolase domain containing 3 | 2.49 | 0.0242 | |
| Bt.7172.1.S1 | myelin oligodendrocyte glycoprotein | 3.45 | 0.0052 | |
| Bt.7677.1.S1 | transmembrane protein 59-like | 3.7 | 0.0475 | |
| Bt.8787.1.S1 | adiponectin receptor-1 | 2.6 | 0.0067 | |
| Bt.3410.1.S1 | synaptogyrin 2 | 2.48 | 0.0476 | |
| Endosome | Bt.11002.1.S1 | OCIA domain containing 1 | −4.92 | 0.0299 |
| Bt.11329.1.S1 | vacuolar protein sorting 11 homolog | 2.41 | 0.0385 | |
| Bt.22508.1.S1 | PRA1 domain family, member 2 | 3.09 | 0.0483 | |
| Others | Bt.12906.1.S1 | similar to Gelsolin precursor (Actin-depolymerizing factor) | 2.59 | 0.0209 |
| Bt.13321.1.S1 | centrosome and spindle pole associated protein 1 | 2.26 | 0.0304 | |
| Bt.14136.1.A1 | similar to Endonuclease domain containing 1 | 3.52 | 0.0386 | |
| Bt.21008.1.S1 | similar to FGFR-like protein | 2.76 | 0.0416 | |
| Bt.22605.1.A1 | zinc finger, CW type with PWWP domain 1 | 2.08 | 0.0178 | |
| Bt.23348.2.S1 | zyxin | 3.83 | 0.0385 | |
| Bt.26865.1.S1 | Myosin head domain containing 1 | 5.75 | 0.0485 | |
| Bt.1409.1.S1 | tubulin polymerization-promoting protein family member 3 | 2.04 | 0.0236 | |
| Bt.4386.1.S1 | synapsin I | 4.24 | 0.0482 | |
| Bt.1088.1.S1 | GTPase, IMAP family member 7 | 0.32 | 0.0419 | |
| Bt.6989.1.S1 | responsive to centrifugal force and shear | 2.79 | 0.007 | |
| Bt.28035.1.S1 | fat storage-inducing transmembrane protein 2 | 3.64 | 0.0367 |
Gene functions are defined largely according to Affymetrix GO biological process term or GO molecular function term.
*: genes associated with the endoplasmic reticulum in bold.
Only 18 genes (8%) were down-regulated and 212 (92%) genes were up-regulated after the repeated or un-annotated probe sets were removed (Table 1). Each step of filtering was re-examined to determine the number of up and down-regulated genes. The 2 fold change filter yielded 2138 probe sets: 792 (37%) of them were down-regulated in BSE field cases and 1346 (63%) probe sets were up-regulated. When the 2 fold change and 1-way ANOVA filters were combined, 409 probe sets were selected: 366 (89%) of them up-regulated and 43 (11%) probe sets down-regulated. Therefore, the up-regulated genes were increased in percentage after the ANOVA filter.
The largest functional group amongst the 230 identified genes was the genes involved in transport (39 genes), followed by the membrane protein group (25 genes), the metabolism group (20 genes) and the DNA and RNA binding group (19 genes; Table 1). The maximal increase was 5.75 fold for Myosin head domain containing 1 and the maximal decrease was 4.92 fold for OCIA domain containing 1.
Many genes in Table 1 were linked to prion diseases in previous studies, such as cathepsin D [12], cathepsin B [13], Inositol 1,4,5-triphosphate receptor [13], apolipoprotein D [13], vimentin [12], [13], heat shock protein 70 [14], transferrin [15], reticulum 1 [16], reticulum 3 [17], a gene similar to solute carrier family 25 [13], CD9 [13], [18], vacuolar protein sorting 11 homolog [11] and DnaJ [11].
The microarray data were validated and confirmed by quantitative PCR using 5 genes: CD47, DnaJ, Hsp70 (up-regulated) and KCNB2, TNFRSF5 (down-regulated) (Figure S1).
Clustering analysis using the 409 probe sets showed that the samples were divided into two groups, Group A contained only negative control samples, while Group B contained all the BSE infected samples plus one negative control sample (Figure 1). This analysis confirmed that the samples of BSE and controls were relatively homogeneous amongst themselves with regard to the genes defined as differentially regulated.
Figure 1. Condition tree of clustering analysis to test tissue sample consistence.
The analysis was performed by GeneSpring using 409 differential regulated probe sets on Bovine GeneChips. The similarity was measured using the Spearman correlation with value 1 for separation ratio and value 0.001 for minimum distance in merge similar branches. N: negative controls and P: clinical BSE samples. Each of coloured bars represents a gene and the colour represents the levels of expression. The relative levels of expression are displayed in different colours: Red: 5; orange: 2; yellow: 1; dark yellow: 0.7; dark blue: 0.4; blue: 0.1.
ER stress is implicated in disease pathogenesis
There were 17 differentially regulated genes whose products are associated with the ER (in bold in Table 1). Upregulation of glucose-regulated protein 94 (Grp94/gp96; ER stress response chaperone) and glucose-regulated protein 170 (Grp170/Orp150; ER stress response chaperone) suggests ER stress [19] as both of them are also known as ER stress markers (Table 1) [20]. Disturbance in the ER leads to ER stress which can be caused by accumulation of unfolded proteins and by changes in calcium homeostasis within the ER [21]. In BSE, many other stress related genes whose products are located in the ER were also up-regulated, such as Inositol 1,4,5-triphosphate receptor (IP3-R; ER calcium-depletion stress) [22]. reticulon 1 (ER stress induced apoptosis) [23], reticulon 3 (ER stress response) [24], reticulon 4 (ER stress induced apoptosis) [25], CDC91 cell division cycle 91-like (Gab1; oxidative stress) [26], procollagen-proline, 2-oxoglutarate 4-dioxygenase (P4HA1; ER stress response) [27], LAG1 homolog, ceramide synthase 2 (CerS2; inhibition of the unfolded protein response and autophagy) [28] and signal sequence receptor, alpha (SSR1 calcium binding) [29] (Table 1). In this study, both cytosolic chaperones Hsp70 and DnaJ were also found up-regulated (Table 1) and this chaperone pair is also induced by ER stress [30]. Other ER stress related gene products in the cytosol were: N-myc downstream regulated gene 1 (Ndrg1; ER stress responsive) [31], aldo-keto reductase family 1, member B1 (Akr1b1; anti ER stress) [32], O-linked N-acetylglucosamine (GlcNAc) transferase (anti ER stress) [33], transketolase (anti ER stress) [34] and cyclin-dependent kinase 5 (Cdk5; Apoptosis in ER stress) [35] (Table 1). These changes suggest the involvement of ER stress during BSE pathogenesis.
In response to ER stress, the unfolded protein response (UPR) is induced to restore cell function by reduction in newly translated proteins entering into the ER, by an increase in the capacity for protein folding [36]. If ER stress is prolonged, the UPR signaling pathways also initiate apoptosis [36]. In BSE, up-regulation of chaperones Grp94 and Grp170 suggests the induction of the UPR; while up-regulation of CerS2 indicates the inhibition of the UPR. To further explore the involvement of ER stress in the pathogenesis of BSE, Western blotting analysis on two more ER stress markers, Grp78 and Chop, was carried out. Grp78, is an ER chaperone and also known as an ER stress master regulator; while Chop is a transcription factor for induction of apoptosis, often up-regulated in response to ER stress [36]. In BSE, the Grp78 protein was up-regulated (Figure 2). Up-regulation of these ER chaperones: Grp78, 94 and 170 indicates the presence of ER stress and the activation of the UPR. The level of Chop was slightly decreased (Figure 2) and this is consistent with the evidence that apoptosis plays a very limited role in BSE [8].
Figure 2. Western blotting of ER stress related proteins Grp78 and Chop.
The relative quantity was the mean values of three controls (N5, N21 and N25) and three clinical BSE samples (P6, P10 and P14). β-Actin was used for normalization. *: p = 0.042 (student's t-test).
Using the gene expression profiles as a biomarker to represent BSE
In our previous BSE time course study, 205 differentially regulated probe sets (corresponding to 114 genes) have been used to show that preclinical animals at 45 months post inoculation (mpi) cluster with cases positive for BSE and allowed the prediction that they are indeed preclinical and close to developing BSE [11]. The same 205 probes sets were used here in a clustering analysis to classify the disease status of the samples from the BSE field cases (Figure 3). These samples fell into two main groups: Group A contained 11 positives and one negative, Group B contained the remaining 11 negatives and three positives. This analysis was therefore able to classify the samples according to infection status with 78.5% (11/14) sensitivity and 92% (11/12) specificity.
Figure 3. Clustering analysis of sample status in the BSE field case study.
The analysis was performed by GeneSpring using 205 differential regulated probe sets generated from the time course study [11]. The similarity was measured using the spearman correlation. N: BSE negative controls; P: clinical BSE samples.
In a reverse analysis, the 409 probe sets identified in this study were used for clustering the samples from the time course study [11]. One group included the negatives, the samples from animals 6 mpi and 36 mpi and the other group contained the positives, and the samples from 21, 27 and 39 mpi animals (Figure 4a). The clustering was similar to the one derived with the 205 probe sets from the time course study [11]. When these 409 probe sets were used to predict the status of the preclinical animals at 45 mpi in the time course study the clustering analysis grouped the individual samples into two groups: one with all the negatives (n = 3) and 6 mpi samples (n = 3) and the other with all the positives (n = 3) and 45 mpi samples (n = 2) (Figure 4b).
Figure 4. Clustering analysis of sample status in the BSE time course study.
The analysis was performed by GeneSpring using 409 differential regulated probe sets generated from this study and the samples were from the BSE time course study [11]. The similarity was measured using the spearman correlation. Neg: BSE negative controls; Pos: clinical BSE samples and m: months post inoculation. (a): the samples were grouped to the time point; (b): the individual samples of negative controls, clinical BSE samples, 6 mpi and 45 mpi.
The analyses above indicate that either the genes from the time course study or the field case samples could be used to predict the infection status. However, it would not be practical to apply all 409 or 205 probe sets as biomarkers to represent BSE. A group of 10 genes were sought to represent BSE from these 230 genes listed in Table 1. Initially, the search was carried out using genes associated with prion diseases (10 genes), ER stress (10 genes), the largest fold changes (10 genes) or the smallest p values (10 genes) separately but the sensitivity and specificity of prediction were low. When these 40 genes were combined and10 genes were selected from them by comparing the expression levels of individual samples from both this study (clinical BSE, n = 14; control, n = 12) and the time course study (clinical BSE, n = 3; control, n = 3), only two groups were produced (Figure 5a). Group A contained all the clinical BSE samples from both studies and group B all the negatives with only three exceptions: P19, Neg2 and Neg3. The sensitivity of these biomarkers was 94% (16/17) and the specificity was 87% (13/15).
Figure 5. Clustering analysis of possible biomarkers for BSE.
The analysis was performed by GeneSpring using 10 differential regulated genes generated from this study. The similarity was measured using the change correlation with value 1 for separation ratio and value 0.001 for minimum distance in merge similar branches. (a), All samples. N: BSE negative controls and P: clinical BSE samples in this study. Pos: clinical BSE and Neg: the negatives from the BSE time course study [11]. (b), samples from the BSE time course study. m: months post inoculation. Each of coloured bars represents a gene and colours represent the levels of expression. The relative levels of expression are displayed in different colours: Red: 5; orange: 2; yellow: 1; dark yellow: 0.7; dark blue: 0.4; blue: 0.1.
These 10 genes above were then used to classify the preclinical samples from the time course study with clustering analysis. The clustering analysis produced two groups: three negatives and three 6 mpi samples being one group and three positives and 45 mpi samples being the other with 100% (5/5) sensitivity and 100% (6/6) specificity (Figure 5b). Therefore, the results of these analyses suggest that these 10 genes might be used to represent the patterns of BSE gene expression at the terminal stages of BSE.
Discussion
In this study, 230 genes were found to be differentially regulated between BSE field cases and controls (Table 1). These genes belong to many functional groups from apoptosis to transport. Seventeen genes were associated with the ER and 10 of them may be involved in stress related situations, especially up-regulation of ER chaperones Grp94 and Grp170 as they are ER stress markers. Since ER stress triggers the UPR [37], [38], [39], the level of protein expression of Grp78, another ER stress marker, was increased in BSE. Up-regulation of Grp78, Grp94 and Grp170 is induced by ER stress response transcription factors XBP1 and ATF6 as all three of them have an ER stress response element (ERSE) in their regulatory regions [36]. These analyses suggest the presence of ER stress and the activation of the UPR in the disease process of BSE. This is in agreement with increasing evidence of the involvement of ER stress in prion diseases [40], [41], [42]. In this study only changes in gene and protein expression of these chaperones were measured to indicate activation of the UPR. There are other methods to measure the induction of the UPR as many proteins are activated or inactivated through phosphorylation cascade in the UPR signalling pathways. For example, the release of Grp78 bound to PERK triggers autophosphorylation of PERK which in turn phosphorylates elf2α to attenuate protein translation [36].
To cope with accumulation of misfolded proteins, ER stress induces ER associated protein degradation I (ERAD I, ubiquitin/proteasome) [43] and ERAD II (autophagy/lysosome) [44], possibly through the UPR. ERAD I is closely linked to the ER quality control system [45] as unfolded or misfolded proteins are targeted for degradation after the failed attempt of folding by ER chaperones. In BSE, ubiquitin-activating enzyme E1 (UBE1) and three E3 ligases: WW domain containing E3 ubiquitin protein ligase 2 [46], ariadne homolog 2 [47] and ubiquitin carboxyl-terminal esterase L1 [48] were found to be up-regulated (Table 1). Recently, the E3 ligase HECTD2 has been identified as genetically associated with vCJD and kuru [49].
ERAD II is also known as autophagy. It is a pathway of self-degradation of cellular components in which autophagosomes sequester organelles or protein aggregates and fuse with lysosomes for degradation. When the production of misfolded proteins exceeds the capacity of ER chaperones and ERAD I, misfolded and aggregated proteins are targeted by the aggresome-autophagy pathway [50]. In BSE, up-regulation of several genes (Table 1) suggests that this pathway might be induced. In the lysosome, both cathepsin B and D (lysosomal hydroases) were up-regulated [44]. On the membrane of the lysosome, the increased levels of lysosomal-associated membrane protein 2 (LAMP2) suggest autophagy initiation [51]. In the cytosol, there were also several up-regulated genes related to ERAD II, such as ubiquitin carboxyl-terminal esterase L1 (aggresome initiation in proteasome inhibition) [48], sphingomyelin phosphodiesterase 1, acid lysosomal (SMPD1; autophagy promotion) [52] and vimentin (cytoskeleton) [14] (Table 1). This association between ERAD II and BSE has been shown in both mice and cattle [53], [54].
In this study, the analyses suggest that ER stress might be involved in BSE pathogenesis and that the UPR, ERAD I and II might all be activated in a concerted effort to rid the cell of harmful PrPSc. The question, therefore, is how much these ER related pathogenic events contribute to fatal prion diseases in general. When the GPI anchor of the PrP protein is removed, the transgenic mice infected with scrapie, also a prion disease, can survive up to 400–600 days post infection (dpi) without clinical scrapie, while the wild type controls develop clinical signs within 140–160 dpi [55]. Some animals with this anchorless PrP have up to 40% more PrPSc than clinically sick controls. The results indicate that infectivity (PrPSc accumulation) and toxicity can be uncoupled. One model to explain it is intra neuronal generation of a toxic intermediate [32]. Here we offer another explanation of prion neurotoxicity using ER stress. The reason for PrPSc accumulation in the ER is because the ER quality control system senses the misfolded forms of PrP and ER chaperones retain them in the ER for folding or degradation by ERAD I. PrPSc is protease resistant so that the rate of removing the misfolded protein is slow; while more and more PrPC converts to PrPSc. Eventually, PrPSc accumulation causes ER stress and the subsequent activation of the UPR and ERAD I and II. Prolonged ER stress leads to cell death [45], [56]. Hence, ER stress related responses might be the major source of prion toxicity. What happens when misfolded PrPSc bypasses the ER quality control? There are lines of evidence that the anchorless prion protein is not detected by the ER quality control system [57], [58]. As the anchorless PrPSc can pass the ER efficiently, there is no toxicity to cause clinical scrapie. Since the cell is not under ER stress, the ERAD pathways are not activated. As a result, more PrPSc accumulates in the brain of transgenic mice with anchorless PrP than in the brain of the wild type controls.
Both the current field case study and the previous time course study were carried out with brainstem tissues infected with BSE [11]. Although these two sets of samples differed in age, in infectious dose and in stages of disease development, many differentially regulated genes were expected to be shared between these two studies. Nonetheless, when the two gene lists were compared, there were only two genes overlapping. However, the profiles generated from one study could be used to predict the sample status of the other study as biomarkers, suggesting that there were some underlying links between these two gene lists (Figures 3 and 4). One possible explanation is that there are more differentially regulated genes than those identified by the analytical method. In order to define a gene list that is relevant with a condition or a disease within a study, the p value is often set at 0.05 or less. However, by doing so, much of the coverage is lost and many differentially regulated genes are not considered. In order to make the list more manageable, an additional 2 fold change filter was introduced to reduce the number of probe sets to 409. If the fold change filter had not been introduced and the p value had been set at 0.1, the number of probe sets would have been 1604. By definition, only 160 of them were selected randomly and the rest of 1446 probe sets should be truly differentially regulated. The remaining 1037 (1446-409) probe sets were not analyzed. Figure 6 provides a simple graphical model for this situation. The small inner circles (stringent settings) overlap only marginally. If all differentially regulated genes had been considered (large circles), there would have been many genes shared by these two studies and that is the most likely reason why the profiles from one study could be used to predict sample status from the other study. In recent years, there have been many publications on gene expression analyses of prion diseases. It is a surprise that relatively few differentially regulated genes are shared between these studies [11], [12], [13], [16], [59], [60]. However, the explanation above for the BSE studies may also apply to gene expression studies of prion diseases in general.
Figure 6. A model to explain the relationship between two BSE gene expression studies.
The larger circles represent all differentially genes; while the inner circles represent differentially regulated genes listed in the studies with p value being less than 0.05. The blue circles: the time course study. The red circles: the field case study.
Considerable efforts have been made to find biomarkers for the prion diseases, especially in the early stage of the incubation period. To date, the detection of PrPres is still the only reliable method. There are some reported potential biomarkers for the disease such as 14-3-3 protein [61], galectin-3 [62], SCRG1 [63], clusterin [64] and cystatin C [65]. However, none of them has been developed for routine diagnosis. One of the reasons may be the natural variation for the single marker within a population. Clustering analysis suggested that a prediction could be made by comparing the gene expression profiles of a sample with those of known BSE positive and negative samples. The analysis also showed a proof of principle that a prediction for a given sample could be made with high sensitivity (94%) and specificity (87%) using just 10 genes as biomarkers although the tissues used in this study were from the brainstem which may not be suitable for diagnose. These ten gene markers might represent the diseased state better than any single markers as they might allow some variations in expression. In Huntington's disease, gene expression profiling of blood reveals a subset of 12 up-regulated mRNAs which have been shown to be able to distinguish controls, presymptomatic Huntington's disease gene carriers and symptomatic Huntington's disease patients [66].
In conclusion, gene expression analysis suggests that BSE infection caused ER stress and the UPR, ERAD I and II might be induced in response to ER stress. Clustering analysis showed that the differentially regulated genes could be used to predict infection status. Ten genes were selected to represent gene expression state in BSE, which might eventually be used as biomarkers.
Materials and Methods
Tissue samples
Brainstem tissues from 100 confirmed cases of BSE in cattle were supplied by the TSE archive at the Veterinary Laboratories Agency, UK. The animals were females, between 4 and 10 years old that had been diagnosed clinically and killed on farm. The major breed was Holstein/Friesian and other breeds were: Limousin Cross, Guernsey, Hereford Cross and Brown Swiss. The negative controls (100 brainstem tissue samples) were from LGC Forensics (Queens Road, Teddington, Middlesex, TW11 0LY, UK) and were comparable in breed, sex and age with the naturally infected BSE samples. Since all samples were from the Archives, approval from the Ethics Committee was not necessary.
Microarrays analysis
The preparations of samples and reagents were carried out according to the Affymetrix GeneChip Expression Analysis manual and as described in the previous study [11]. The RNA samples were resolved by 1% agarose gels and selected according to the integrity of ribosomal RNA bands. Since the tissues used in this study were from cattle naturally infected with BSE (field cases), the quality of RNA was generally poor. From 100 cases each, the best quality RNA samples, 12 controls and 14 BSE infected, were selected for microarray analysis with Affymetrix GeneChip Bovine Genome Arrays. The raw data were first imported into the Affymetrix GeneChip operating software version 1.4. All array data were MIAME compliant and the raw data were deposited in ArrayExpress with the accession number: E-MTAB-302. After initial analysis, the pivot formatted data were further analysed with the GeneSpring version 7 software (Silicon Genetics). The data were normalized in three steps: 1. Data transformation set measurements less than 0.01 to 0.01; 2. Each measurement was divided by the 50.0th percentile of all measurements in that sample; 3. Each measurement for each gene in test samples was divided by the median of that gene's measurements in the corresponding control samples. The value for each gene was divided by the median of its measurements in all samples. If the median of the raw values was below 10 then each measurement for that gene was divided by 10. If the numerator was above 10, the measurement was discarded. These steps were the default settings for the GeneSpring package.
Two filters were used to find differently regulated genes: 2 fold change and the one way ANOVA statistical analysis with the parameters of 0.05 for p-value cutoff, multiple testing correction and Student-Newman-Keuls for the post hoc tests, without assume variances equal for the parametric test.
Western blotting
Cell-free extracts (60 µg protein) were loaded on 12% 1-D SDS PAGE (Invitrogen) and resolved proteins from several mini-gels were transferred to the same PVDF membrane (Millipore) so that one set of samples was used to monitor protein loading using β-Actin. The blots were immuno-stained with mouse monoclonal anti-β-Actin IgG (Santa Cruz Biotech), rabbit polyclonal anti-Grp78 (US Biological) and rabbit polyclonal anti-Chop (BioLegend). The protein bands were visualized by using secondary antibodies, alkaline phosphatase conjugated IgGs (anti-mouse, Santa Cruz Biotech; anti-rabbit, Sigma) and the ECL developer kit (Amersham). The images were captured by Fluor-S MultiImager (Bio-Rad) and the protein bands were quantified by the Quantity One software (Bio-Rad).
Quantitative PCR
The RNA samples were treated with the DNA free™ kit (Ambion) for 1 h at 37°C to remove any trace of DNA. The treated RNA was then used as a template for cDNA synthesis with the TaqMan reverse transcription kit (Applied Biosystems). The real time PCR was carried out by denaturing at 95°C for 15 s, annealing at 50°C for 2 min and extension at 60°C for 1 min for 40 cycles using an ABI Prism 7700 Sequencing Detector. The GAPDH gene was used as an internal control to normalize the expression levels of target mRNA. The primer sets were chosen by the Primer Express 1.5 for TaqMan software. The sequences of the primer sets were as following: for CD47, 5′-TCC ATT AAC GAT TCT AAA TAA AGG AAA CT, 5′-TGC TAT GGA AAA AAG CCC CC and the probe, FAM-5′-TGG TGT TGC TAT GCG TGA GAT CCT CTC C; for DNAJ, 5′-TCT GTG AAA ATA AAG CAG GAG TGA A, 5′- AGT GAG AAA CAG CCA AAA TAC TGA AC and the probe, FAM-5′- CCT TTG CAG ACT TCA GAC TGG TTG GAT TTC; for KCNB2, 5′- TGA TGA CTT CTT AGA GCT CCA GGG, 5′-CAA GCA GTT TGG GCT GGA GT and the probe, FAM-5′-AGG AGG CCG GAC AAG CAG GCA; for HS70, 5′- GGA CTT TGG TCT TGC CCT ATA TTT AC, 5′-CAC ACT CAC TAT AAC ATA CAG AAA TAA CA AAA A and the probe, FAM-5′-TGT GAT GTG TCA GTT TGT TCT ATG ATA AGG TTG TAA TCT C; for TNFRSF5, 5′-CGT GGA GAC GAT TGA TCC G, 5′- AGC ATA AGG TCT CTT GCA CCG and the probe, FAM-5′- AGG ATT TTC CCG GCC CCC ACC.
Supporting Information
Validation of microarray data by RT-PCR. 1 and 2: CD47; 3 and 4: DNAJ; 5 and 6: KCNB; 7 and 8: HS70; 9 and 10: TNFRSF5. The values of gene expression are listed at the top for comparison. No fill: negative controls; Grey: clinical BSE.
(0.24 MB TIF)
Unannotated probe sets in the BSE field case study
(0.18 MB DOC)
Acknowledgments
We thank Dr T. Haferlach and Leukemia Diagnostics, Ludwig-Maximilians University, Munich, Germany for the use of the Affymextrix workstation. Thanks also to Dr Martin Jeffrey for insightful comments on the manuscript and to Mrs Sharon Everitt for Western blotting analysis.
Footnotes
Competing Interests: The authors have declared that no competing interests exist.
Funding: This work was supported by a development grant of Veterinary Laboratories Agency UK. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
References
- 1.Prusiner SB. Prions. Proc Natl Acad Sci U S A. 1998;95:13363–13383. doi: 10.1073/pnas.95.23.13363. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 2.Ironside JW. Neuropathological findings in new variant CJD and experimental transmission of BSE. FEMS Immunol Med Microbiol. 1998;21:91–95. doi: 10.1111/j.1574-695X.1998.tb01153.x. [DOI] [PubMed] [Google Scholar]
- 3.Wells GAH, Wilesmith JW. Chapter 12: Bovine Spongiform Encephalopathy and Related Diseases. In: Prusiner SB, editor. Prion Biology and Diseases. New York: Spring Harbor Laboratory Press; 2004. pp. 595–628. [Google Scholar]
- 4.Jeffrey M, Gonzalez L, Espenes A, Press CM, Martin S, et al. Transportation of prion protein across the intestinal mucosa of scrapie-susceptible and scrapie-resistant sheep. J Pathol. 2006;209:4–14. doi: 10.1002/path.1962. [DOI] [PubMed] [Google Scholar]
- 5.Wells GA, Scott AC, Johnson CT, Gunning RF, Hancock RD, et al. A novel progressive spongiform encephalopathy in cattle. Vet Rec. 1987;121:419–420. doi: 10.1136/vr.121.18.419. [DOI] [PubMed] [Google Scholar]
- 6.Wilesmith JW, Ryan JB, Atkinson MJ. Bovine spongiform encephalopathy: epidemiological studies on the origin. Vet Rec. 1991;128:199–203. doi: 10.1136/vr.128.9.199. [DOI] [PubMed] [Google Scholar]
- 7.Bruce ME, Will RG, Ironside JW, McConnell I, Drummond D, et al. Transmissions to mice indicate that ‘new variant’ CJD is caused by the BSE agent. Nature. 1997;389:498–501. doi: 10.1038/39057. [DOI] [PubMed] [Google Scholar]
- 8.Theil D, Fatzer R, Meyer R, Schobesberger M, Zurbriggen A, et al. Nuclear DNA fragmentation and immune reactivity in bovine spongiform encephalopathy. J Comp Pathol. 1999;121:357–367. doi: 10.1053/jcpa.1999.0333. [DOI] [PubMed] [Google Scholar]
- 9.Capobianco R, Casalone C, Suardi S, Mangieri M, Miccolo C, et al. Conversion of the BASE Prion Strain into the BSE Strain: The Origin of BSE? PLoS Pathog. 2007;3:e31. doi: 10.1371/journal.ppat.0030031. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 10.Gavier-Widen D, Stack MJ, Baron T, Balachandran A, Simmons M. Diagnosis of transmissible spongiform encephalopathies in animals: a review. J Vet Diagn Invest. 2005;17:509–527. doi: 10.1177/104063870501700601. [DOI] [PubMed] [Google Scholar]
- 11.Tang Y, Xiang W, Hawkins SA, Kretzschmar HA, Windl O. Transcriptional changes in the brains of cattle orally infected with the bovine spongiform encephalopathy agent precede detection of infectivity. J Virol. 2009;83:9464–9473. doi: 10.1128/JVI.00352-09. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 12.Xiang W, Windl O, Wunsch G, Dugas M, Kohlmann A, et al. Identification of differentially expressed genes in scrapie-infected mouse brains by using global gene expression technology. J Virol. 2004;78:11051–11060. doi: 10.1128/JVI.78.20.11051-11060.2004. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 13.Skinner PJ, Abbassi H, Chesebro B, Race RE, Reilly C, et al. Gene expression alterations in brains of mice infected with three strains of scrapie. BMC Genomics. 2006;7:114. doi: 10.1186/1471-2164-7-114. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 14.Kristiansen M, Messenger MJ, Klohn PC, Brandner S, Wadsworth JD, et al. Disease-related prion protein forms aggresomes in neuronal cells leading to caspase activation and apoptosis. J Biol Chem. 2005;280:38851–38861. doi: 10.1074/jbc.M506600200. [DOI] [PubMed] [Google Scholar]
- 15.Singh A, Mohan ML, Isaac AO, Luo X, Petrak J, et al. Prion protein modulates cellular iron uptake: a novel function with implications for prion disease pathogenesis. PLoS One. 2009;4:e4468. doi: 10.1371/journal.pone.0004468. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 16.Booth S, Bowman C, Baumgartner R, Dolenko B, Sorensen G, et al. Molecular classification of scrapie strains in mice using gene expression profiling. Biochem Biophys Res Commun. 2004;325:1339–1345. doi: 10.1016/j.bbrc.2004.10.150. [DOI] [PubMed] [Google Scholar]
- 17.Brown AR, Rebus S, McKimmie CS, Robertson K, Williams A, et al. Gene expression profiling of the preclinical scrapie-infected hippocampus. Biochem Biophys Res Commun. 2005;334:86–95. doi: 10.1016/j.bbrc.2005.06.060. [DOI] [PubMed] [Google Scholar]
- 18.Doh-ura K, Mekada E, Ogomori K, Iwaki T. Enhanced CD9 expression in the mouse and human brains infected with transmissible spongiform encephalopathies. J Neuropathol Exp Neurol. 2000;59:774–785. doi: 10.1093/jnen/59.9.774. [DOI] [PubMed] [Google Scholar]
- 19.Kamauchi S, Nakatani H, Nakano C, Urade R. Gene expression in response to endoplasmic reticulum stress in Arabidopsis thaliana. FEBS J. 2005;272:3461–3476. doi: 10.1111/j.1742-4658.2005.04770.x. [DOI] [PubMed] [Google Scholar]
- 20.Sharma NK, Das SK, Mondal AK, Hackney OG, Chu WS, et al. Endoplasmic reticulum stress markers are associated with obesity in nondiabetic subjects. J Clin Endocrinol Metab. 2008;93:4532–4541. doi: 10.1210/jc.2008-1001. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 21.Lindholm D, Wootz H, Korhonen L. ER stress and neurodegenerative diseases. Cell Death Differ. 2006;13:385–392. doi: 10.1038/sj.cdd.4401778. [DOI] [PubMed] [Google Scholar]
- 22.Kuo TH, Liu BF, Yu Y, Wuytack F, Raeymaekers L, et al. Co-ordinated regulation of the plasma membrane calcium pump and the sarco(endo)plasmic reticular calcium pump gene expression by Ca2+. Cell Calcium. 1997;21:399–408. doi: 10.1016/s0143-4160(97)90051-8. [DOI] [PubMed] [Google Scholar]
- 23.Fazi B, Melino S, De Rubeis S, Bagni C, Paci M, et al. Acetylation of RTN-1C regulates the induction of ER stress by the inhibition of HDAC activity in neuroectodermal tumors. Oncogene. 2009;28:3814–3824. doi: 10.1038/onc.2009.233. [DOI] [PubMed] [Google Scholar]
- 24.Wan Q, Kuang E, Dong W, Zhou S, Xu H, et al. Reticulon 3 mediates Bcl-2 accumulation in mitochondria in response to endoplasmic reticulum stress. Apoptosis. 2007;12:319–328. doi: 10.1007/s10495-006-0574-y. [DOI] [PubMed] [Google Scholar]
- 25.Kuang E, Wan Q, Li X, Xu H, Zou T, et al. ER stress triggers apoptosis induced by Nogo-B/ASY overexpression. Exp Cell Res. 2006;312:1983–1988. doi: 10.1016/j.yexcr.2006.02.024. [DOI] [PubMed] [Google Scholar]
- 26.Holgado-Madruga M, Wong AJ. Gab1 is an integrator of cell death versus cell survival signals in oxidative stress. Mol Cell Biol. 2003;23:4471–4484. doi: 10.1128/MCB.23.13.4471-4484.2003. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 27.Vonk LA, Doulabi BZ, Huang CL, Helder MN, Everts V, et al. Endoplasmic reticulum stress inhibits collagen synthesis independent of collagen-modifying enzymes in different chondrocyte populations and dermal fibroblasts. Biochem Cell Biol. 2010;88:539–552. doi: 10.1139/o09-174. [DOI] [PubMed] [Google Scholar]
- 28.Spassieva SD, Mullen TD, Townsend DM, Obeid LM. Disruption of ceramide synthesis by CerS2 down-regulation leads to autophagy and the unfolded protein response. Biochem J. 2009;424:273–283. doi: 10.1042/BJ20090699. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 29.Wada I, Rindress D, Cameron PH, Ou WJ, Doherty JJ, 2nd, et al. SSR alpha and associated calnexin are major calcium binding proteins of the endoplasmic reticulum membrane. J Biol Chem. 1991;266:19599–19610. [PubMed] [Google Scholar]
- 30.Okushima Y, Koizumi N, Yamaguchi Y, Kimata Y, Kohno K, et al. Isolation and characterization of a putative transducer of endoplasmic reticulum stress in Oryza sativa. Plant Cell Physiol. 2002;43:532–539. doi: 10.1093/pcp/pcf063. [DOI] [PubMed] [Google Scholar]
- 31.Agarwala KL, Kokame K, Kato H, Miyata T. Phosphorylation of RTP, an ER stress-responsive cytoplasmic protein. Biochem Biophys Res Commun. 2000;272:641–647. doi: 10.1006/bbrc.2000.2833. [DOI] [PubMed] [Google Scholar]
- 32.Keith RJ, Haberzettl P, Vladykovskaya E, Hill BG, Kaiserova K, et al. Aldose reductase decreases endoplasmic reticulum stress in ischemic hearts. Chem Biol Interact. 2009;178:242–249. doi: 10.1016/j.cbi.2008.10.055. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 33.Ngoh GA, Hamid T, Prabhu SD, Jones SP. O-GlcNAc signaling attenuates ER stress-induced cardiomyocyte death. Am J Physiol Heart Circ Physiol. 2009;297:H1711–1719. doi: 10.1152/ajpheart.00553.2009. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 34.Tan SX, Teo M, Lam YT, Dawes IW, Perrone GG. Cu, Zn superoxide dismutase and NADP(H) homeostasis are required for tolerance of endoplasmic reticulum stress in Saccharomyces cerevisiae. Mol Biol Cell. 2009;20:1493–1508. doi: 10.1091/mbc.E08-07-0697. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 35.Saito T, Konno T, Hosokawa T, Asada A, Ishiguro K, et al. p25/cyclin-dependent kinase 5 promotes the progression of cell death in nucleus of endoplasmic reticulum-stressed neurons. J Neurochem. 2007;102:133–140. doi: 10.1111/j.1471-4159.2007.04540.x. [DOI] [PubMed] [Google Scholar]
- 36.Lai E, Teodoro T, Volchuk A. Endoplasmic reticulum stress: signaling the unfolded protein response. Physiology (Bethesda) 2007;22:193–201. doi: 10.1152/physiol.00050.2006. [DOI] [PubMed] [Google Scholar]
- 37.Ryu EJ, Harding HP, Angelastro JM, Vitolo OV, Ron D, et al. Endoplasmic reticulum stress and the unfolded protein response in cellular models of Parkinson's disease. J Neurosci. 2002;22:10690–10698. doi: 10.1523/JNEUROSCI.22-24-10690.2002. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 38.Lisbona F, Hetz C. Turning off the unfolded protein response: an interplay between the apoptosis machinery and ER stress signaling. Cell Cycle. 2009;8:1643–1644. [PubMed] [Google Scholar]
- 39.Lindenmeyer MT, Rastaldi MP, Ikehata M, Neusser MA, Kretzler M, et al. Proteinuria and hyperglycemia induce endoplasmic reticulum stress. J Am Soc Nephrol. 2008;19:2225–2236. doi: 10.1681/ASN.2007121313. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 40.Ferreiro E, Costa R, Marques S, Cardoso SM, Oliveira CR, et al. Involvement of mitochondria in endoplasmic reticulum stress-induced apoptotic cell death pathway triggered by the prion peptide PrP(106-126). J Neurochem. 2008;104:766–776. doi: 10.1111/j.1471-4159.2007.05048.x. [DOI] [PubMed] [Google Scholar]
- 41.Hetz C, Russelakis-Carneiro M, Maundrell K, Castilla J, Soto C. Caspase-12 and endoplasmic reticulum stress mediate neurotoxicity of pathological prion protein. Embo J. 2003;22:5435–5445. doi: 10.1093/emboj/cdg537. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 42.Hetz C, Russelakis-Carneiro M, Walchli S, Carboni S, Vial-Knecht E, et al. The disulfide isomerase Grp58 is a protective factor against prion neurotoxicity. J Neurosci. 2005;25:2793–2802. doi: 10.1523/JNEUROSCI.4090-04.2005. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 43.Sundar Rajan S, Srinivasan V, Balasubramanyam M, Tatu U. Endoplasmic reticulum (ER) stress & diabetes. Indian J Med Res. 2007;125:411–424. [PubMed] [Google Scholar]
- 44.He C, Klionsky DJ. Regulation mechanisms and signaling pathways of autophagy. Annu Rev Genet. 2009;43:67–93. doi: 10.1146/annurev-genet-102808-114910. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 45.Groenendyk J, Michalak M. Endoplasmic reticulum quality control and apoptosis. Acta Biochim Pol. 2005;52:381–395. [PubMed] [Google Scholar]
- 46.Bates PW, Vierstra RD. UPL1 and 2, two 405 kDa ubiquitin-protein ligases from Arabidopsis thaliana related to the HECT-domain protein family. Plant J. 1999;20:183–195. doi: 10.1046/j.1365-313x.1999.00590.x. [DOI] [PubMed] [Google Scholar]
- 47.Marteijn JA, van der Meer LT, van Emst L, van Reijmersdal S, Wissink W, et al. Gfi1 ubiquitination and proteasomal degradation is inhibited by the ubiquitin ligase Triad1. Blood. 2007;110:3128–3135. doi: 10.1182/blood-2006-11-058602. [DOI] [PubMed] [Google Scholar]
- 48.Lehman NL. The ubiquitin proteasome system in neuropathology. Acta Neuropathol. 2009;118:329–347. doi: 10.1007/s00401-009-0560-x. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 49.Lloyd SE, Maytham EG, Pota H, Grizenkova J, Molou E, et al. HECTD2 is associated with susceptibility to mouse and human prion disease. PLoS Genet. 2009;5:e1000383. doi: 10.1371/journal.pgen.1000383. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 50.Chin LS, Olzmann JA, Li L. Parkin-mediated ubiquitin signalling in aggresome formation and autophagy. Biochem Soc Trans. 2010;38:144–149. doi: 10.1042/BST0380144. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 51.Eskelinen EL, Tanaka Y, Saftig P. At the acidic edge: emerging functions for lysosomal membrane proteins. Trends Cell Biol. 2003;13:137–145. doi: 10.1016/s0962-8924(03)00005-9. [DOI] [PubMed] [Google Scholar]
- 52.Patschan S, Chen J, Polotskaia A, Mendelev N, Cheng J, et al. Lipid mediators of autophagy in stress-induced premature senescence of endothelial cells. Am J Physiol Heart Circ Physiol. 2008;294:H1119–1129. doi: 10.1152/ajpheart.00713.2007. [DOI] [PubMed] [Google Scholar]
- 53.Ersdal C, Goodsir CM, Simmons MM, McGovern G, Jeffrey M. Abnormal prion protein is associated with changes of plasma membranes and endocytosis in bovine spongiform encephalopathy (BSE)-affected cattle brains. Neuropathol Appl Neurobiol. 2009;35:259–271. doi: 10.1111/j.1365-2990.2008.00988.x. [DOI] [PubMed] [Google Scholar]
- 54.Jeffrey M, Scott JR, Williams A, Fraser H. Ultrastructural features of spongiform encephalopathy transmitted to mice from three species of bovidae. Acta Neuropathol. 1992;84:559–569. doi: 10.1007/BF00304476. [DOI] [PubMed] [Google Scholar]
- 55.Chesebro B, Trifilo M, Race R, Meade-White K, Teng C, et al. Anchorless prion protein results in infectious amyloid disease without clinical scrapie. Science. 2005;308:1435–1439. doi: 10.1126/science.1110837. [DOI] [PubMed] [Google Scholar]
- 56.Rao RV, Ellerby HM, Bredesen DE. Coupling endoplasmic reticulum stress to the cell death program. Cell Death Differ. 2004;11:372–380. doi: 10.1038/sj.cdd.4401378. [DOI] [PubMed] [Google Scholar]
- 57.Winklhofer KF, Heske J, Heller U, Reintjes A, Muranyi W, et al. Determinants of the in vivo folding of the prion protein. A bipartite function of helix 1 in folding and aggregation. J Biol Chem. 2003;278:14961–14970. doi: 10.1074/jbc.M209942200. [DOI] [PubMed] [Google Scholar]
- 58.Ashok A, Hegde RS. Selective processing and metabolism of disease-causing mutant prion proteins. PLoS Pathog. 2009;5:e1000479. doi: 10.1371/journal.ppat.1000479. [DOI] [PMC free article] [PubMed] [Google Scholar]
- 59.Xiang W, Hummel M, Mitteregger G, Pace C, Windl O, et al. Transcriptome analysis reveals altered cholesterol metabolism during the neurodegeneration in mouse scrapie model. J Neurochem. 2007;102:834–847. doi: 10.1111/j.1471-4159.2007.04566.x. [DOI] [PubMed] [Google Scholar]
- 60.Sawiris GP, Becker KG, Elliott EJ, Moulden R, Rohwer RG. Molecular analysis of bovine spongiform encephalopathy infection by cDNA arrays. J Gen Virol. 2007;88:1356–1362. doi: 10.1099/vir.0.82387-0. [DOI] [PubMed] [Google Scholar]
- 61.Collins S, Boyd A, Fletcher A, Gonzales M, McLean CA, et al. Creutzfeldt-Jakob disease: diagnostic utility of 14-3-3 protein immunodetection in cerebrospinal fluid. J Clin Neurosci. 2000;7:203–208. doi: 10.1054/jocn.1999.0193. [DOI] [PubMed] [Google Scholar]
- 62.Jin JK, Na YJ, Song JH, Joo HG, Kim S, et al. Galectin-3 expression is correlated with abnormal prion protein accumulation in murine scrapie. Neurosci Lett. 2007;420:138–143. doi: 10.1016/j.neulet.2007.04.069. [DOI] [PubMed] [Google Scholar]
- 63.Dron M, Bailly Y, Beringue V, Haeberle AM, Griffond B, et al. Scrg1 is induced in TSE and brain injuries, and associated with autophagy. Eur J Neurosci. 2005;22:133–146. doi: 10.1111/j.1460-9568.2005.04172.x. [DOI] [PubMed] [Google Scholar]
- 64.Sasaki K, Doh-ura K, Ironside J, Mabbott N, Iwaki T. Clusterin expression in follicular dendritic cells associated with prion protein accumulation. J Pathol. 2006;209:484–491. doi: 10.1002/path.2009. [DOI] [PubMed] [Google Scholar]
- 65.Sanchez JC, Guillaume E, Lescuyer P, Allard L, Carrette O, et al. Cystatin C as a potential cerebrospinal fluid marker for the diagnosis of Creutzfeldt-Jakob disease. Proteomics. 2004;4:2229–2233. doi: 10.1002/pmic.200300799. [DOI] [PubMed] [Google Scholar]
- 66.Borovecki F, Lovrecic L, Zhou J, Jeong H, Then F, et al. Genome-wide expression profiling of human blood reveals biomarkers for Huntington's disease. Proc Natl Acad Sci U S A. 2005;102:11023–11028. doi: 10.1073/pnas.0504921102. [DOI] [PMC free article] [PubMed] [Google Scholar]
Associated Data
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Supplementary Materials
Validation of microarray data by RT-PCR. 1 and 2: CD47; 3 and 4: DNAJ; 5 and 6: KCNB; 7 and 8: HS70; 9 and 10: TNFRSF5. The values of gene expression are listed at the top for comparison. No fill: negative controls; Grey: clinical BSE.
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Unannotated probe sets in the BSE field case study
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