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Signature^®LTx Leukemia Translocation Panel v2.0 (RUO)*

4 Diseases • 9 Translocations • 12 Fusion Transcripts • 1 Well

Use Signature^® LTx v2.0 for the rapid detection and identification of the fusion transcripts from common chromosome translocations/abnormalities associated with CML, ALL, APL and AML*. Signature^® LTx v2.0 utilizes both multiplex RT-PCR and automated multiplex detection on the Luminex^® 100^™ IS or 200^™ System.

Signature^® LTx v2.0 provides comprehensive information in a single well reducing the need for and cost of maintaining and training on numerous platforms and assays.

Figure 1. Overview of the Signature LTx v2.0 assay principle and workflow (click to enlarge).

Signature^® LTx v2.0 has a simple workflow that requires minimal hands-on time. The assay contains a single transfer step of amplified products directly to the bead mix, without intervening purifications. The average time to results is approximately 6 hours for up to 24 reactions per kit.

Table 2: Simultaneous Detection of 12 Leukemia-Associated Fusion Transcripts and Endogenous Control GAPDH^† (click to enlarge).

Signature^® LTx Negative, Positive and No Target (NTC) controls were analyzed together with 400 ng of total RNA specimens purified from 8 different translocation positive leukemic cell lines. Qualitative results are measured by MFI (mean fluorescent intensity). MFI values greater than or equal to 350 MFI signify positive detection for a specific fusion transcript. A sample is considered negative if the MFI value is below 350 MFI and the GAPDH signal is greater than or equal to 1,000 MFI. Specific fusion transcripts were detected in specimens undiluted (100%) or diluted 1:100 (1%) into a background of 400 ng of translocation negative leukemic cell line RNA (HL-60). This analytical sensitivity is equivalent to the detection of 1 fusion transcript positive cell in a background of at least 100 fusion transcript negative cells. No cross reactivity between the various targets was observed and MFI values for all non-target probes were reproducibly below the cut-off (350 MFI).

Figure 2: Serial Dilution of Cell line total RNA^† (click to enlarge).

Fusion transcripts were prepared by in vitro transcription (IVT) and spiked into a background of total RNA purified from a translocation negative leukemic cell line. In this experiment, 4 different IVT RNAs were serially diluted into a constant background of 400 ng of HL-60 total RNA. Only MFI results for PML/RARα (L or S form), inv(16) type D, MLL/AF4 (e10/e4) and the GAPDH probes are shown. Each fusion transcript target was detected specifically in specimens containing 2x10⁶, 2x10⁵ or 2x10⁴ copies (labeled 2M, 200K and 20K respectively in the figure). The MFI obtained for the fusion transcripts and the endogenous control GAPDH transcript were in the same range as those obtained with cell line RNA specimens.

Attributes for Signature® LTx* v2.0:

^* Research Use Only. Not intended for use in diagnostic procedures.

^† Preliminary research data, the performance characteristics of this assay are not yet established.

References

Gabert J, Beillard E, van der Velden VH, Bi W, Grimwade D, Pallisgaard N, Barbany G, Cazzaniga G, Cayuela JM, Cave H, Pane F, Aerts JL, De Micheli D, Thirion X, Pradel V, Gonzalez M, Viehmann S, Malec M, Saglio G, van Dongen JJ. Standardization and Quality Control Studies of “Real-Time” Quantitative reverse Transcriptase Polymerase Chain Reaction of Fusion Gene Transcripts for Residual Disease Detection in Leukemia – A Europe Against Cancer Program. Leukemia. 17(12):2318-57. 2003.

Salto-Tellez M, Shelat SG, Benoit B, Rennert H, Carroll M, Leonard DG, Nowell P, Bagg A. Multiplex RT-PCR for the Detection of Leukemia-Associated Translocations: Validation and Application to Routine Molecular Diagnostic Practice. J Mol Diagn. 5(4):231-6. 2003.

Bock O, Reising D, Kreipe H. Multipilex RT-PCR for the Detection of Common BCR-ABL Fusion Transcripts in Paraffin-Embedded Tissues from Patients with Chronic Myeloid Leukemia and Acute Lymphoblastic Leukemia. Diagn Mol Pathol. 12(3):119-23. 2003.

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