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Center for Computational Systems Medicine
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Fusion Gene and Fusion Protein Summary

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Fusion Amino Acid Sequences (multiple BPs and multiple gene isoforms)

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Fusion Protein Breakpoint Sequences - (for the Screening of the FusionNeoAntigens)

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Potential FusionNeoAntigens in HLA I - (netMHCpan v4.1 + deepHLApan v1.1)

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Potential FusionNeoAntigens in HLA II - (netMHCIIpan v4.1)

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Fusion Breakpoint 14 AA Peptide Structure - (RoseTTAFold)

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Filtering FusionNeoAntigens Through Checking the Interaction with HLAs in 3D - (Glide)

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Vaccine Design for the FusionNeoAntigens (RNA/protein sequences)

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Potential target of CAR-T therapy development

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Information on the samples that have these potential fusion neoantigens

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Fusion Protein Targeting Drugs - (Manual Curation)

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Fusion Protein Related diseases - (Manual Curation)

Fusion Protein:CYP2E1-AMACR

Fusion Gene and Fusion Protein Summary

check button Fusion gene summary
Fusion partner gene informationFusion gene name: CYP2E1-AMACR
FusionPDB ID: 21055
FusionGDB2.0 ID: 21055
HgeneTgene
Gene symbol

CYP2E1

AMACR

Gene ID

1571

23600

Gene namecytochrome P450 family 2 subfamily E member 1alpha-methylacyl-CoA racemase
SynonymsCPE1|CYP2E|P450-J|P450C2EAMACRD|CBAS4|P504S|RACE|RM
Cytomap

10q26.3

5p13.2

Type of geneprotein-codingprotein-coding
Descriptioncytochrome P450 2E14-nitrophenol 2-hydroxylaseCYPIIE1cytochrome P450, family 2, subfamily E, polypeptide 1cytochrome P450, subfamily IIE (ethanol-inducible), polypeptide 1cytochrome P450-Jflavoprotein-linked monooxygenasemicrosomal monooxygenasexealpha-methylacyl-CoA racemase2-methylacyl-CoA racemase
Modification date2020031520200313
UniProtAcc

P05181

Main function of 5'-partner protein: FUNCTION: A cytochrome P450 monooxygenase involved in the metabolism of fatty acids (PubMed:10553002, PubMed:18577768). Mechanistically, uses molecular oxygen inserting one oxygen atom into a substrate, and reducing the second into a water molecule, with two electrons provided by NADPH via cytochrome P450 reductase (NADPH--hemoprotein reductase) (PubMed:10553002, PubMed:18577768). Catalyzes the hydroxylation of carbon-hydrogen bonds. Hydroxylates fatty acids specifically at the omega-1 position displaying the highest catalytic activity for saturated fatty acids (PubMed:10553002, PubMed:18577768). May be involved in the oxidative metabolism of xenobiotics (Probable). {ECO:0000269|PubMed:10553002, ECO:0000269|PubMed:18577768, ECO:0000305|PubMed:9348445}.

Q9UHK6

Main function of 5'-partner protein: FUNCTION: Catalyzes the interconversion of (R)- and (S)-stereoisomers of alpha-methyl-branched-chain fatty acyl-CoA esters (PubMed:7649182, PubMed:10655068, PubMed:11060359). Acts only on coenzyme A thioesters, not on free fatty acids, and accepts as substrates a wide range of alpha-methylacyl-CoAs, including pristanoyl-CoA, trihydroxycoprostanoyl-CoA (an intermediate in bile acid synthesis), and arylpropionic acids like the anti-inflammatory drug ibuprofen (2-(4-isobutylphenyl)propionic acid) but neither 3-methyl-branched nor linear-chain acyl-CoAs (PubMed:7649182, PubMed:10655068, PubMed:11060359). {ECO:0000269|PubMed:10655068, ECO:0000269|PubMed:11060359, ECO:0000269|PubMed:7649182}.
Ensembl transtripts involved in fusion geneENST idsENST00000480558, ENST00000252945, 
ENST00000463117, 		ENST00000335606, 
ENST00000382072, ENST00000382068, 
ENST00000382085, ENST00000426255, 
ENST00000441713, ENST00000502637, 
ENST00000512079, ENST00000514195, 
Fusion gene scores for assessment (based on all fusion genes of FusionGDB 2.0)* DoF score8 X 5 X 3=12028 X 3 X 4=336
# samples 823
** MAII scorelog2(8/120*10)=-0.584962500721156
possibly effective Gene in Pan-Cancer Fusion Genes (peGinPCFGs).
DoF>8 and MAII<0		log2(23/336*10)=-0.546827371834385
possibly effective Gene in Pan-Cancer Fusion Genes (peGinPCFGs).
DoF>8 and MAII<0
Fusion gene context

PubMed: CYP2E1 [Title/Abstract] AND AMACR [Title/Abstract] AND fusion [Title/Abstract]

Fusion neoantigen context

PubMed: CYP2E1 [Title/Abstract] AND AMACR [Title/Abstract] AND neoantigen [Title/Abstract]

Most frequent breakpoint (based on all fusion genes of FusionGDB 2.0)CYP2E1(135342144)-AMACR(34006004), # samples:1
Anticipated loss of major functional domain due to fusion event.CYP2E1-AMACR seems lost the major protein functional domain in Hgene partner, which is a CGC by not retaining the major functional domain in the partially deleted in-frame ORF.
CYP2E1-AMACR seems lost the major protein functional domain in Hgene partner, which is a CGC by not retaining the major functional domain in the partially deleted in-frame ORF.
CYP2E1-AMACR seems lost the major protein functional domain in Hgene partner, which is a essential gene by not retaining the major functional domain in the partially deleted in-frame ORF.
CYP2E1-AMACR seems lost the major protein functional domain in Hgene partner, which is a essential gene by not retaining the major functional domain in the partially deleted in-frame ORF.
* DoF score (Degree of Frequency) = # partners X # break points X # cancer types
** MAII score (Major Active Isofusion Index) = log2(# samples/DoF score*10)

check button Gene ontology of each fusion partner gene with evidence of Inferred from Direct Assay (IDA) from Entrez
PartnerGeneGO IDGO termPubMed ID
HgeneCYP2E1

GO:0002933

lipid hydroxylation

10553002

HgeneCYP2E1

GO:0016098

monoterpenoid metabolic process

16401082

HgeneCYP2E1

GO:0017144

drug metabolic process

19219744

HgeneCYP2E1

GO:0018960

4-nitrophenol metabolic process

9348445

HgeneCYP2E1

GO:0046483

heterocycle metabolic process

19651758

HgeneCYP2E1

GO:0055114

oxidation-reduction process

16401082|19219744

TgeneAMACR

GO:0008206

bile acid metabolic process

10655068



check button Four levels of functional features of fusion genes
Go to FGviewer search page for the most frequent breakpoint (https://ccsmweb.uth.edu/FGviewer/chr10:135342144/chr5:34006004)
- FGviewer provides the online visualization of the retention search of the protein functional features across DNA, RNA, protein, and pathological levels.
- How to search
1. Put your fusion gene symbol.
2. Press the tab key until there will be shown the breakpoint information filled.
4. Go down and press 'Search' tab twice.
4. Go down to have the hyperlink of the search result.
5. Click the hyperlink.
6. See the FGviewer result for your fusion gene.
FGviewer

check buttonRetention analysis results of each fusion partner protein across 39 protein features of UniProt such as six molecule processing features, 13 region features, four site features, six amino acid modification features, two natural variation features, five experimental info features, and 3 secondary structure features, are available here.

check buttonFusion gene breakpoints across CYP2E1 (5'-gene)
* Click on the image to open the UCSC genome browser with custom track showing this image in a new window.
all structure

check buttonFusion gene breakpoints across AMACR (3'-gene)
* Click on the image to open the UCSC genome browser with custom track showing this image in a new window.
all structure


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Fusion Amino Acid Sequences


check buttonFusion information from ORFfinder translation from full-length transcript sequence from FusionPDB.
HenstTenstHgeneHchrHbpHstrandTgeneTchrTbpTstrandSeq length
(transcript)		BP loci
(transcript)		Predicted start
(transcript)		Predicted stop
(transcript)		Seq length
(amino acids)
ENST00000463117CYP2E1chr10135342144+ENST00000335606AMACRchr534006004-44266092001510436
ENST00000463117CYP2E1chr10135342144+ENST00000382072AMACRchr534006004-3269609200958252
ENST00000252945CYP2E1chr10135342144+ENST00000335606AMACRchr534006004-4187370331271412
ENST00000252945CYP2E1chr10135342144+ENST00000382072AMACRchr534006004-303037033719228

check buttonDeepORF prediction of the coding potential based on the fusion transcript sequence of in-frame fusion genes. DeepORF is a coding potential classifier based on convolutional neural network by comparing the real Ribo-seq data. If the no-coding score < 0.5 and coding score > 0.5, then the in-frame fusion transcript is predicted as being likely translated.
HenstTenstHgeneHchrHbpHstrandTgeneTchrTbpTstrandNo-coding scoreCoding score
ENST00000463117ENST00000335606CYP2E1chr10135342144+AMACRchr534006004-0.0002880960.99971193
ENST00000463117ENST00000382072CYP2E1chr10135342144+AMACRchr534006004-0.0398366380.9601633
ENST00000252945ENST00000335606CYP2E1chr10135342144+AMACRchr534006004-8.25E-050.9999175
ENST00000252945ENST00000382072CYP2E1chr10135342144+AMACRchr534006004-0.0047440160.995256

check button Predicted full-length fusion amino acid sequences. For individual full-length fusion transcript sequence from FusionPDB, we ran ORFfinder and chose the longest ORF among all the predicted ones.

Get the fusion protein sequences from here.

Fusion protein sequence information is available in the fasta format.
>FusionGDB ID_FusionGDB isoform ID_FGname_Hgene_Hchr_Hbp_Henst_Tgene_Tchr_Tbp_Tenst_length(fusion AA) seq_BP

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Fusion Protein Breakpoint Sequences for CYP2E1-AMACR

check button +/-13 AA sequence from the breakpoints of the fusion protein sequences.
HgeneHchrHbpTgeneTchrTbpLength(fusion protein)BP in fusion proteinPeptide
CYP2E1chr10135342144AMACRchr534006004370112RGDLPAFHAHRDRGVMEKLQLGPEIL
CYP2E1chr10135342144AMACRchr534006004609136RGDLPAFHAHRDRGVMEKLQLGPEIL

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Potential FusionNeoAntigen Information of CYP2E1-AMACR in HLA I

check button Multiple sequence alignments of the potential FusionNeoAntigens per fusion breakpoints. If the MSA is empty, then it means that there were predicted fusion neoantigens in this fusion breakpoint, but those predicted fusion neoantigens were not across the breakpoint, which is not fusion-specific.
CYP2E1-AMACR_135342144_34006004.msa

check button Potential FusionNeoAntigen Information
* We used NetMHCpan v4.1 (%rank<0.5) and deepHLApan v1.1 (immunogenic score>0.5)
Fusion geneHchrHbpTgeneTchrTbpHLA IFusionNeoAntigen peptideBinding scoreImmunogenic scoreNeoantigen start (at BP 13)Neoantigen end (at BP 13)
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:05HRDRGVMEK0.98810.8444918
CYP2E1-AMACRchr10135342144chr534006004370HLA-B47:01RDRGVMEKL0.17240.62531019
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:07HRDRGVMEKL0.99690.5392919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:01HRDRGVMEKL0.98390.7434919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B38:01HRDRGVMEKL0.96330.8354919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B38:02HRDRGVMEKL0.95820.8323919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B07:10HRDRGVMEKL0.54040.6564919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B07:10AHRDRGVMEKL0.86790.7516819
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:14HRDRGVMEK0.9760.8449918
CYP2E1-AMACRchr10135342144chr534006004370HLA-C12:12HAHRDRGVM0.88620.9028716
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:03HRDRGVMEK0.6760.8613918
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:09HRDRGVMEKL0.99010.6487919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:12HRDRGVMEKL0.97890.7516919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:05HRDRGVMEKL0.96490.7232919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:10HRDRGVMEK0.98260.865918
CYP2E1-AMACRchr10135342144chr534006004370HLA-B15:09FHAHRDRGV0.80780.5108615
CYP2E1-AMACRchr10135342144chr534006004370HLA-C16:01HAHRDRGVM0.57520.9539716
CYP2E1-AMACRchr10135342144chr534006004370HLA-B48:05RDRGVMEKL0.06770.55161019
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:09HRDRGVMEKL0.99740.7093919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B27:06HRDRGVMEKL0.99720.7272919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:31HRDRGVMEKL0.98520.7461919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B38:05HRDRGVMEKL0.96330.8354919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B39:11HRDRGVMEKL0.88890.6721919
CYP2E1-AMACRchr10135342144chr534006004370HLA-B15:09FHAHRDRGVM0.88790.6507616

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Potential FusionNeoAntigen Information of CYP2E1-AMACR in HLA II

check button Multiple sequence alignments of the potential FusionNeoAntigens per fusion breakpoints. If the MSA is empty, then it means that there were predicted fusion neoantigens in this fusion breakpoint, but those predicted fusion neoantigens were not across the breakpoint, which is not fusion-specific.
CYP2E1-AMACR_135342144_34006004.msa

check button Potential FusionNeoAntigen Information
* We used NetMHCIIpan v4.1 (%rank<0.5).
Fusion geneHchrHbpTgeneTchrTbpHLA IIFusionNeoAntigen peptideNeoantigen start (at BP 13)Neoantigen end (at BP 13)
CYP2E1-AMACRchr10135342144chr534006004370DRB1-1367LPAFHAHRDRGVMEK318
CYP2E1-AMACRchr10135342144chr534006004370DRB1-1515LPAFHAHRDRGVMEK318

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Fusion breakpoint peptide structures of CYP2E1-AMACR

check button3D structures of the fusion breakpoint peptide of 14AA sequence that have potential fusion neoantigens
* The minimum length of the amino acid sequence in RoseTTAFold is 14AA. Here, we predicted the 14AA fusion protein breakpoint sequence not the fusion neoantigen peptide, which is shorter than 14 AA.
File nameBPseqHgeneTgeneHchrHbpTchrTbpAAlen
2392FHAHRDRGVMEKLQCYP2E1AMACRchr10135342144chr534006004370

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Filtering FusionNeoAntigens Through Checking the Interaction with HLAs in 3D of CYP2E1-AMACR

check buttonVirtual screening between 25 HLAs (from PDB) and FusionNeoAntigens
* We used Glide to predict the interaction between HLAs and neoantigens.
HLA allelePDB IDFile nameBPseqDocking scoreGlide score
HLA-B14:023BVN2392FHAHRDRGVMEKLQ-7.9962-8.1096
HLA-B14:023BVN2392FHAHRDRGVMEKLQ-5.70842-6.74372
HLA-B52:013W392392FHAHRDRGVMEKLQ-6.83737-6.95077
HLA-B52:013W392392FHAHRDRGVMEKLQ-4.4836-5.5189
HLA-A11:014UQ22392FHAHRDRGVMEKLQ-10.0067-10.1201
HLA-A11:014UQ22392FHAHRDRGVMEKLQ-9.03915-10.0745
HLA-A24:025HGA2392FHAHRDRGVMEKLQ-6.56204-6.67544
HLA-A24:025HGA2392FHAHRDRGVMEKLQ-5.42271-6.45801
HLA-B44:053DX82392FHAHRDRGVMEKLQ-7.85648-8.89178
HLA-B44:053DX82392FHAHRDRGVMEKLQ-5.3978-5.5112
HLA-A02:016TDR2392FHAHRDRGVMEKLQ-3.37154-4.40684

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Vaccine Design for the FusionNeoAntigens of CYP2E1-AMACR

check button mRNA and peptide sequences of FusionNeoAntigens that have potential interaction with HLA-Is.
Fusion geneHchrHbpTchrTbpStart in +/-13AAEnd in +/-13AAFusionNeoAntigen peptide sequenceFusionNeoAntigen RNA sequence
CYP2E1-AMACRchr10135342144chr5340060041019RDRGVMEKLGGGACAGGGGTGTCATGGAGAAACTCC
CYP2E1-AMACRchr10135342144chr534006004615FHAHRDRGVTCCATGCGCACAGGGACAGGGGTGTCA
CYP2E1-AMACRchr10135342144chr534006004616FHAHRDRGVMTCCATGCGCACAGGGACAGGGGTGTCATGG
CYP2E1-AMACRchr10135342144chr534006004716HAHRDRGVMATGCGCACAGGGACAGGGGTGTCATGG
CYP2E1-AMACRchr10135342144chr534006004819AHRDRGVMEKLCGCACAGGGACAGGGGTGTCATGGAGAAACTCC
CYP2E1-AMACRchr10135342144chr534006004918HRDRGVMEKACAGGGACAGGGGTGTCATGGAGAAAC
CYP2E1-AMACRchr10135342144chr534006004919HRDRGVMEKLACAGGGACAGGGGTGTCATGGAGAAACTCC

check button mRNA and peptide sequences of FusionNeoAntigens that have potential interaction with HLA-IIs.
Fusion geneHchrHbpTchrTbpStart in +/-13AAEnd in +/-13AAFusionNeoAntigen peptideFusionNEoAntigen RNA sequence
CYP2E1-AMACRchr10135342144chr534006004318LPAFHAHRDRGVMEKTCCCCGCGTTCCATGCGCACAGGGACAGGGGTGTCATGGAGAAAC

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Information of the samples that have these potential fusion neoantigens of CYP2E1-AMACR

check button These samples were reported as having these fusion breakpoints. For individual breakpoints, we checked the open reading frames considering multiple gene isoforms and chose the in-frame fusion genes only. Then, we made fusion protein sequences and predicted the fusion neoantigens. These fusion-positive samples may have these potential fusion neoantigens.
Cancer typeFusion geneHchrHbpHenstTchrTbpTenstSample
LIHCCYP2E1-AMACRchr10135342144ENST00000252945chr534006004ENST00000335606TCGA-DD-A39W-01A

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Potential target of CAR-T therapy development for CYP2E1-AMACR

check button Predicted 3D structure. We used RoseTTAFold.

check buttonRetention analysis result of each fusion partner protein across 39 protein features of UniProt such as six molecule processing features, 13 region features, four site features, six amino acid modification features, two natural variation features, five experimental info features, and 3 secondary structure features. Here, to provide the retention of the transmembrane domain, we only show the protein feature retention information of those transmembrane features


* Minus value of BPloci means that the break point is located before the CDS.
- In-frame and retained 'Transmembrane'.
PartnerGeneHbpTbpENSTStrandBPexonTotalExonProtein feature loci*BPlociTotalLenProtein featureProtein feature note

check button Subcellular localization prediction of the transmembrane domain retained fusion proteins
* We used DeepLoc 1.0. The order of the X-axis of the barplot is as follows: Entry_ID, Localization, Type, Nucleus, Cytoplasm, Extracellular, Mitochondrion, Cell_membrane, Endoplasmic_reticulum, Plastid, Golgi.apparatus, Lysosome.Vacuole, Peroxisome. Y-axis is the output score of DeepLoc. Clicking the image will open a new tab with a large image.
HgeneHchrHbpHenstTgeneTchrTbpTenstDeepLoc result

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Related Drugs to CYP2E1-AMACR

check button Drugs used for this fusion-positive patient.
(Manual curation of PubMed, 04-30-2022 + MyCancerGenome)
HgeneTgeneDrugSourcePMID

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Related Diseases to CYP2E1-AMACR

check button Diseases that have this fusion gene.
(Manual curation of PubMed, 04-30-2022 + MyCancerGenome)
HgeneTgeneDiseaseSourcePMID

check button Diseases associated with fusion partners.
(DisGeNet 4.0)
PartnerGeneDisease IDDisease name# pubmedsSource