S7710
TRAPeze™ RT Telomerase Detection Kit
A highly sensitive in vitro assay for the fluorometric detection & real time quantification of telomerase activity in cells.
Synonym(s):
TRAP Assay
Sign In to View Organizational & Contract Pricing.
Select a Size
About This Item
UNSPSC Code:
12161503
NACRES:
NA.32
eCl@ss:
32161000
Product Name
TRAPeze™ RT Telomerase Detection Kit, A highly sensitive in vitro assay for the fluorometric detection & real time quantification of telomerase activity in cells.
manufacturer/tradename
Chemicon®
TRAPeze™
application(s)
genomic analysis
shipped in
dry ice
Quality Level
General description
Telomeres are specific structures found at the end of chromosomes in eukaryotes. In human chromosomes, the telomeres consist of thousands of copies of 6 base repeats (TTAGGG)(1-3). It has been suggested that telomeres protect chromosome ends since damaged chromosomes lacking telomeres undergo fusion, rearrangement and translocation (2). In somatic cells, telomere length is progressively shortened with each cell division both in vivo and in vitro (4-7) due to the inability of the DNA polymerase complex to synthesize the very 5′ end of the lagging strand (8,9).
Telomerase is a ribonucleoprotein that synthesizes and directs the telomeric repeats onto the 3′ end of existing telomeres using its RNA component as a template (10-14). Telomerase activity has been shown to be specifically expressed in immortal cells, cancer and germ cells (15,16) where it compensates for telomere shortening during DNA replication and thus stabilizes telomere length (7,17). These observations have led to a hypothesis that telomere length may function as a "mitotic clock" to sense the number of cell divisions and eventually signal replicative senescence or programmed cell death when a critical telomere length is achieved. Therefore, expression of telomerase activity in cancer cells may be a necessary and essential step for tumor development and progression (16,18-20). The causal relationship between expression of telomerase and telomere length stabilization and the extension of the life span of the human cell has recently been reported (21).
The development of a sensitive and efficient PCR-based telomerase activity detection method, TRAP (Telomeric Repeat Amplification Protocol) (15, 22), has made possible large scale surveys of telomerase activity in human cells and tissues (15, 23-29). To date, telomerase activity has been detected in over 85% of all tumors tested spanning more than 20 different types of cancers (30-31).
The TRAPeze™ RT Telomerase Detection Kit is a highly sensitive in vitro assay for the fluorometric detection and real time quantification of telomerase activity. It incorporates refinements to the original TRAP assay that were first introduced in the gel-based TRAPeze™ Telomerase Detection Kit (Cat. No. S7700) and adds the ability to quantitate telomerase activity using fluorescence energy transfer (ET) primers similar to the TRAPeze™ XL Telomerase Detection Kit (Cat. No. S7707). As in the original TRAPeze™ Kit, primer sequence modifications that reduce amplification artifacts and PCR controls for standard curve generation are included. In addition, both the TRAPeze™ RT and XL Kits use fluorescence energy transfer (ET) primers to generate fluorescently labeled TRAP products which permit nonisotopic, quantitative analysis of telomerase activity.
The unique design of these ET primers (Amplifluor® primers) allows detection and quantification of telomerase activity by directly measuring real time fluorescence emission in the reaction vessels. Since Amplifluor® primers will fluoresce only upon incorporation into the TRAP products, post-PCR sample manipulations such as electrophoretic gel or ELISA analyses are eliminated, thereby reducing the the risk of carry-over contamination. Quantitative analysis is not compromised when detection is performed in a high-throughput 96-well format unlike platforms utilizing a qualitative ELISA. Additionaly, an additional stand alone control is provided separately to assess PCR inhibitors that may be present in experimental samples. (Please see product insert for references).
Telomerase is a ribonucleoprotein that synthesizes and directs the telomeric repeats onto the 3′ end of existing telomeres using its RNA component as a template (10-14). Telomerase activity has been shown to be specifically expressed in immortal cells, cancer and germ cells (15,16) where it compensates for telomere shortening during DNA replication and thus stabilizes telomere length (7,17). These observations have led to a hypothesis that telomere length may function as a "mitotic clock" to sense the number of cell divisions and eventually signal replicative senescence or programmed cell death when a critical telomere length is achieved. Therefore, expression of telomerase activity in cancer cells may be a necessary and essential step for tumor development and progression (16,18-20). The causal relationship between expression of telomerase and telomere length stabilization and the extension of the life span of the human cell has recently been reported (21).
The development of a sensitive and efficient PCR-based telomerase activity detection method, TRAP (Telomeric Repeat Amplification Protocol) (15, 22), has made possible large scale surveys of telomerase activity in human cells and tissues (15, 23-29). To date, telomerase activity has been detected in over 85% of all tumors tested spanning more than 20 different types of cancers (30-31).
The TRAPeze™ RT Telomerase Detection Kit is a highly sensitive in vitro assay for the fluorometric detection and real time quantification of telomerase activity. It incorporates refinements to the original TRAP assay that were first introduced in the gel-based TRAPeze™ Telomerase Detection Kit (Cat. No. S7700) and adds the ability to quantitate telomerase activity using fluorescence energy transfer (ET) primers similar to the TRAPeze™ XL Telomerase Detection Kit (Cat. No. S7707). As in the original TRAPeze™ Kit, primer sequence modifications that reduce amplification artifacts and PCR controls for standard curve generation are included. In addition, both the TRAPeze™ RT and XL Kits use fluorescence energy transfer (ET) primers to generate fluorescently labeled TRAP products which permit nonisotopic, quantitative analysis of telomerase activity.
The unique design of these ET primers (Amplifluor® primers) allows detection and quantification of telomerase activity by directly measuring real time fluorescence emission in the reaction vessels. Since Amplifluor® primers will fluoresce only upon incorporation into the TRAP products, post-PCR sample manipulations such as electrophoretic gel or ELISA analyses are eliminated, thereby reducing the the risk of carry-over contamination. Quantitative analysis is not compromised when detection is performed in a high-throughput 96-well format unlike platforms utilizing a qualitative ELISA. Additionaly, an additional stand alone control is provided separately to assess PCR inhibitors that may be present in experimental samples. (Please see product insert for references).
The TRAPeze™ RT Telomerase Detection Kit is a highly sensitive in vitro assay for the fluorometric detection and real time quantification of telomerase activity. It incorporates refinements to the original TRAPeze™ assay and adds the ability to quantitate telomerase activity using fluorescence energy transfer (ET) primers.
Other Notes
CHAPS Lysis Buffer (13.5mL)
5X TRAPeze™ RT Reaction Mix (1.12mL)
5X TRAPeze™ Control Reaction Mix (1.12mL)
PCR - Grade Water (8.2mL)
TSR8* (quantitation control template) (45 μL)
TSK* (pcr inhibition/normalization control) (45 μL)
Control Cell Pellet (Telomerase positive cells; 106 cells)
* Caution - refer to Sec. II. Kit Components, Precautions in product insert.
5X TRAPeze™ RT Reaction Mix (1.12mL)
5X TRAPeze™ Control Reaction Mix (1.12mL)
PCR - Grade Water (8.2mL)
TSR8* (quantitation control template) (45 μL)
TSK* (pcr inhibition/normalization control) (45 μL)
Control Cell Pellet (Telomerase positive cells; 106 cells)
* Caution - refer to Sec. II. Kit Components, Precautions in product insert.
Packaging
The kit provides enough reagents to perform 224 TRAPeze™ RT reactions.
Preparation Note
1. CHAPS Lysis Buffer - 15°C to -25°C
2. 5X TRAPeze™ RT Reaction Mix -15°C to -25°C
3. 5X TRAPeze™ Control Reaction Mix 2°C to 8°C
4. PCR - Grade Water - 15°C to -25°C
5. TSR8 -15°C to -25°C
6. TSK -15°C to -25°C
7. Control Cell Pellet -75°C to -85°C
2. 5X TRAPeze™ RT Reaction Mix -15°C to -25°C
3. 5X TRAPeze™ Control Reaction Mix 2°C to 8°C
4. PCR - Grade Water - 15°C to -25°C
5. TSR8 -15°C to -25°C
6. TSK -15°C to -25°C
7. Control Cell Pellet -75°C to -85°C
Legal Information
Amplifluor is a registered trademark of Merck KGaA, Darmstadt, Germany
CHEMICON is a registered trademark of Merck KGaA, Darmstadt, Germany
TRAPEZE is a trademark of Merck KGaA, Darmstadt, Germany
signalword
Warning
hcodes
Hazard Classifications
Aquatic Chronic 3 - Met. Corr. 1
Storage Class
8B - Non-combustible corrosive hazardous materials
flash_point_f
Not applicable
flash_point_c
Not applicable
Certificates of Analysis (COA)
Search for Certificates of Analysis (COA) by entering the products Lot/Batch Number. Lot and Batch Numbers can be found on a product’s label following the words ‘Lot’ or ‘Batch’.
Already Own This Product?
Find documentation for the products that you have recently purchased in the Document Library.
Stanley T Parish et al.
Journal of immunology (Baltimore, Md. : 1950), 182(7), 4237-4243 (2009-03-21)
Expanded populations of CD8(+) T lymphocytes lacking CD28 expression are associated with a variety of deleterious clinical outcomes, including early mortality in the elderly, more rapid progression to AIDS, cardiovascular disease, and enhanced tumor cell growth. In cell culture, irreversible
Estrogen and telomerase in human peripheral blood mononuclear cells.
Ann L Benko,Nancy J Olsen,William J Kovacs
Molecular and cellular endocrinology null
Sylwia Kabacik et al.
Aging, 10(10), 2800-2815 (2018-10-18)
The paramount role of senescent cells in ageing has prompted suggestions that re-expression of telomerase may prevent ageing; a proposition that is predicated on the assumption that senescent cells are the sole cause of ageing. Recently, several DNA methylation-based age
Cullin 5 regulates cortical layering by modulating the speed and duration of Dab1-dependent neuronal migration.
Sim?? S, Jossin Y, Cooper JA
The Journal of Neuroscience null
A Static Magnetic Field Inhibits the Migration and Telomerase Function of Mouse Breast Cancer Cells.
Zhu Fan et al.
BioMed research international, 2020, 7472618-7472618 (2020-05-29)
Static magnetic field (SMF) has a potential as a cancer therapeutic modality due to its specific inhibitory effects on the proliferation of multiple cancer cells. However, the underlying mechanism remains unclear, and just a few studies have examined the effects
Related Content
"Epigenetics describes heritable changes in gene expression caused by non-genetic mechanisms instead of by alterations in DNA sequence. These changes can be cell- or tissue-specific, and can be passed on to multiple generations. Epigenetic regulation enriches DNAbased information, allowing a cell to vary its response across diverse biological and environmental contexts. Although epigenetic mechanisms are primarily centered in the nucleus, these mechanisms can be induced by environmental signals such as hormones, nutrients, stress, and cellular damage, pointing to the involvement of cytoplasmic and extracellular factors in epigenetic regulation."
Global Trade Item Number
| SKU | GTIN |
|---|---|
| S7710 | 04053252006302 |
Our team of scientists has experience in all areas of research including Life Science, Material Science, Chemical Synthesis, Chromatography, Analytical and many others.
Contact Technical Service