Services

Omics Services

Genomics
Epigenomics
Single Cell/Spatial Omics
Metagenomics
Transcriptomics
Proteomics
Bioinformatics
Pre-made Library
CLIA Lab Services
Clinical Genetic Testing
Capabilities
Resources
Promotions
Support
About Us
Let's Connect
Services

Omics Services

Research Services
Genomics
Epigenomics
Single Cell/Spatial Omics
Metagenomics
Transcriptomics
Clinical Services
CLIA Lab Services
Clinical Genetic Testing
Capabilities
Resources
Promotions
Support
About Us
Let's Connect
CLINICAL CAPABILITIES // Genetic testing

Sarcoma

Identify genetic risk factors and causes of rare cancer.

Clinical at Psomagen

Who Would Benefit from Sarcoma Genetic Testing?

1

A person with a strong family history of certain types of cancer

Determine if they carry a gene mutation that increases their risk. If they do have an inherited mutation, they might want to have screening tests to look for cancer early, or even take steps to try to lower their risk.

2

A person already diagnosed with cancer

This is especially true if there are other factors to suggest the cancer might have been caused by an inherited mutation (such as a strong family history or if the cancer was diagnosed at a young age). Genetic testing might show if the person has a higher risk of developing cancer. It can also help other family members decide if they want to be tested for the mutation.  

3

Family members of a person known to have an inherited gene mutation that increases their risk of cancer

Testing can help them know if they need screening tests to look for cancer early, or if they should take steps to try to lower their risk.

How Do I Order a Test?

A printed copy of the requisition form must be submitted with the specimen if you are not placing your order through the online portal. You can find and print a copy of the requisition form here. If you need to modify your order, please contact client services.

Sarcoma Panel Best Practices

Preferred Specimen

2mL whole blood in a purple-top EDTA tube (K2EDTA or K3EDTA)

Alternate Specimens

  • Saliva
  • Buccal swab
  • gDNA
Let's get started!

How to Ship Your Samples

Follow IATA Regulations

Please note that Psomagen sample collection kits are built to protect the samples from being damaged during transport and to comply with the International Air Transport Association (IATA) regulation. If you are using packaging other than that provided by Psomagen, please make sure to follow the "three layers of packaging" rule to avoid the risk of having the package destroyed by the courier:

  • A primary sample receptacle sealed (collection tube).
  • A leak-proof specimen bag containing absorbent material.
  • An outer packaging that meets the local postal regulations and is labeled as “Exempt Human Specimen.”

For more information please refer to page 187 of IATA Dangerous Goods Regulation.

Additional Shipment Requirements

For saliva, ship at room temperature (overnight shipping is not necessary).

For blood, we recommend using overnight shipping the same day that the blood is collected.

  • Blood can be kept at room temperature for up to 48 hours.
  • We request that blood is refrigerated no longer than two weeks.
  • Please do not freeze blood as deletion/duplication analysis is not supported for frozen or partially frozen blood.

Please ship the specimen in a crush-proof container via FedEx Priority Overnight (in accordance with the FedEx Packaging Guidelines for Clinical Samples.

Our US Shipping Address

Attn: Clinical Laboratory Testing Personnel
Psomagen Inc.
1330 Piccard Drive, Ste 103
Rockville, MD 20850

Test for 22 related genes

Gene List

APC
BLM
CDKN1C
DICER1
EPCAM
FH
HRAS
KIT
MLH1
MSH2
MSH6
NBN
NF1
PDGFRA
PMS2
PRKAR1A
PTCH1
RB1
RECQL4
SDHA
SDHB
SDHC
SDHD
SUFU
TP53
WRN
 

Test Methodology and Limitations

DNA sequencing involves the extraction of genomic DNA from specimens collected in approved containers and provided the specimen meets required sample minimum quantity (e.g. volume, weight, etc). This is followed by quantification and qualification to ensure the adequacy of amount and purity for sequencing. Subsequently, whole exome sequencing is conducted on an IlluminaTM short read sequencing (SRS) platform (e.g., Novaseq X PlusTM) at Psomagen, Inc.’s laboratories (CLIA # 21D2062464, CAP # 8742212).

DNA sequence alignment, variant calling, and variant filtering are performed utilizing the Illumina DRAGENTM bioinformatics pipeline (version 4.2.4.) and various tool sets, which align reads to the human reference genome (GRCh38) and identify single nucleotide variants (SNVs) and small insertions/deletions (InDels). Variant annotations are performed using a pipeline available in Fabric Enterprise. Variant review and interpretation are conducted according to the standards and guidelines set forth by the American College of Medical Genetics and Genomics (Richards S, et al., Genet Med., 2015) by Fabric Clinical Labs (CLIA #45D2281059, CAP # 9619501). Only variants classified as pathogenic or likely pathogenic are reported. The following quality filters are applied to all variants: coverage <40x, allele balance outside 0.3-0.7.

Variants in the following genes are reported: APC, BLM, CDKN1C, DICER1, EPCAM, FH, HRAS, KIT, MLH1, MSH2, MSH6, NBN, NF1, PDGFRA, PMS2, PRKAR1A, PTCH1, RB1, RECQL4, SDHA, SDHB, SDHC, SDHD, SUFU, TP53, WRN.

This test is designed to detect single nucleotide variants (SNVs) and small insertions/deletions (InDels). Next-Generation Sequencing (NGS) coverage may vary across the genome, potentially resulting in missed variants in regions with low coverage depth. Some genetic abnormalities may be undetectable with the current version of this test. While the DRAGEN bioinformatics pipeline demonstrates high accuracy for variant calling, there remains a possibility of false positive or false negative results due to variant interpretation which relies on current scientific knowledge and available databases. This may lead to the reclassification of reported variants as new information emerges from ongoing research and is updated in the ACMG guidelines. Furthermore, systematic chemical, computational, or human errors may contribute to false positives or false negatives of DNA variants. For any reported variants, confirmation by orthogonal technology and subsequent consultation with a genetic counselor or qualified healthcare provider can help to establish definitive risk. This result should be considered preliminary until such confirmation has been performed.

Clinical management for this individual should be based on personal and family history, along with other relevant information. If considered relevant to this individual’s clinical presentation and/or family history, targeted testing of appropriate family members of this individual for the reported variants may help to interpret these results. For assistance with the interpretation of these results, healthcare professionals may contact Psomagen directly at (301) 251-1007 or support@psomagen.com.

More Resources

  1. Bonin SPetrera FRosai JStanta GDNA and RNA obtained from Bouin's fixed tissuesJ. Clin. Pathol. 200558313316.

  2. Hill DAPfeifer JDMarley EF et al. WT1 staining reliably differentiates desmoplastic small round cell tumor from Ewing sarcoma/primitive neuroectodermal tumor. An immunohistochemical and molecular diagnostic studyAm. J. Clin. Pathol. 2000114345353.

  3. Cook JRDehner LPCollins MH et al. Anaplastic lymphoma kinase (ALK) expression in the inflammatory myofibroblastic tumor: a comparative immunohistochemical studyAm. J. Surg. Pathol. 20012513641371.

  4. Cessna MHZhou HSanger WG et al. Expression of ALK1 and p80 in inflammatory myofibroblastic tumor and its mesenchymal mimics: a study of 135 casesMod. Pathol. 200215931938.

  5. Mitelman FJohansson BMertens F (eds). Mitelman Database of Chromosome Aberrations in Cancer (2005). http://cgap.nci.nih.gov/Chromosomes/Mitelman

  6. Rabbitts THChromosomal translocations in human cancerNature 1994372143149.

  7. Rabbitts THPerspective: chromosomal translocations can affect genes controlling gene expression and differentiation—why are these functions targeted? J. Pathol. 19991873942.

  8. Schlessinger JCell signaling by receptor tyrosine kinasesCell 2002103211225.

  9. Knezevich SRMcFadden DETao WLim JFSorensen PHA novel ETV6-NTRK3 gene fusion in congenital fibrosarcomaNat. Genet. 199818184187.

  10. Bourgeois JMKnezevich SRMathers JASorensen PHMolecular detection of the ETV6-NTRK3 gene fusion differentiates congenital fibrosarcoma from other childhood spindle cell tumorsAm. J. Surg. Pathol. 200024937946.

  11. Simon MPPedeutour FSirvent N et al. Deregulation of the platelet-derived growth factor B-chain gene via fusion with collagen gene COL1A1 in dermatofibrosarcoma protuberans and giant-cell fibroblastomaNat. Genet. 1997159598.

  1. Antonescu CRTschernyavsky SJDecuseara Ret al. Prognostic impact of P53 status, TLS-CHOP fusion transcript structure, and histological grade in myxoid liposarcoma: a molecular and clinicopathologic study of 82 cases Cancer Res. 2001739773987.

  2. Waters BLPanagopoulos IAllen EFGenetic characterization of angiomatoid fibrous histiocytoma identifies fusion of the FUS and ATF-1 genes induced by a chromosomal translocation involving bands 12q13 and 16p11Cancer Genet. Cytogenet.2000121109116.

Our Certifications

CLIA ID number: 21D2062464
CAP ID number: 8742212