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Invitrogen™
100 bp DNA Ladder
Invitrogen 100 bp DNA Ladder is designed for sizing and approximate quantification of double-stranded DNA in the range of 100Read more
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| Catalog Number | Quantity |
|---|---|
| 15628019 | 100 Applications |
| 15628050 | 500 Applications |
Catalog number 15628019
Price (CNY)
561.00
Online Exclusive
Ends: 31-Dec-2025
1,927.00Save 1,366.00 (71%)
Each
In stock
Quantity:
100 Applications
Price (CNY)
561.00
Online Exclusive
Ends: 31-Dec-2025
1,927.00Save 1,366.00 (71%)
Each
Invitrogen 100 bp DNA Ladder is designed for sizing and approximate quantification of double-stranded DNA in the range of 100 bp to 2,000 bp. 100 bp DNA Ladder consists of 13 individual chromatography-purified DNA fragments and has reference bands at 2000, 1500, and 600 bp for easy orientation.
100 bp DNA Ladder is ideal for separation on 1–2% agarose gels.
Highlights of 100 bp DNA Ladder:
• Sharp, clear bands—chromatography purified fragments for consistent and reliable results
• Convenient—provided with 10X BlueJuice Gel Loading Buffer for tracking of sample DNA migration
• Precise—an exact amount of DNA in each band
Product use
The double-stranded DNA ladder can be visualized on 1–2% agarose gels after ethidium bromide or SYBR Safe staining. The ladder is designed with a uniform intensity of DNA bands for a clear view of each band. An exact amount of DNA in each band allows approximate quantification of DNA samples.
This ladder can be radiolabeled with T4 polynucleotide kinase or T4 DNA polymerase.
100 bp DNA Ladder is ideal for separation on 1–2% agarose gels.
Highlights of 100 bp DNA Ladder:
• Sharp, clear bands—chromatography purified fragments for consistent and reliable results
• Convenient—provided with 10X BlueJuice Gel Loading Buffer for tracking of sample DNA migration
• Precise—an exact amount of DNA in each band
Product use
The double-stranded DNA ladder can be visualized on 1–2% agarose gels after ethidium bromide or SYBR Safe staining. The ladder is designed with a uniform intensity of DNA bands for a clear view of each band. An exact amount of DNA in each band allows approximate quantification of DNA samples.
This ladder can be radiolabeled with T4 polynucleotide kinase or T4 DNA polymerase.
For Research Use Only. Not for use in diagnostic procedures.
Specifications
Concentration0.5 μg/μL
Gel CompatibilityAgarose gel
Green FeaturesSustainable packaging
Kit Contents100 μL DNA Ladder, 1 mL 10X Sample Loading Buffer, 100 Applications
No. of Reactions100 Applications
Product TypeDNA Ladder
Quantity100 Applications
Ready to LoadNo
Sample Loading Volume1 mL
Shipping ConditionApproved for shipment at Room Temperature or on Dry Ice
TechnologyIndividual chromatography-purified DNA fragments
Volume (Metric)100 μL
Gel TypeAgarose
Size Range100 to 2000 bp
Unit SizeEach
Contents & Storage
• 100 µL 100 bp DNA Ladder
• 1 mL 10X BlueJuice Gel Loading Buffer
Store at -20°C.
• 1 mL 10X BlueJuice Gel Loading Buffer
Store at -20°C.
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100 bp DNA Ladder
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Lot #Certificate TypeDateCatalog Number(s)
3264099Certificate of AnalysisJun 18, 202515628050
3262966Certificate of AnalysisJun 17, 202515628019
3262669Certificate of AnalysisJun 17, 202515628019
3261893Certificate of AnalysisJun 16, 202515628019
3249543Certificate of AnalysisMay 29, 202515628050
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Safety Data Sheets
SDSFrequently asked questions (FAQs)
Sequences of Invitrogen DNA and RNA ladders are proprietary.
Invitrogen DNA ladders contain linear dsDNA fragments.
Invitrogen DNA ladders are composed of double-stranded DNA fragments only.
Here are a few reasons why you might see smearing of the bands:
- The DNA was degraded. Avoid nuclease contamination of DNA standards.
- Too much DNA was loaded on the gel. Decrease the amount of DNA in the gel.
- The DNA was contaminated by protein. Remove proteins by phenol extraction before electrophoresis.
- For small DNA, the bands may have diffused during staining. Add the ethidium bromide before electrophoresis.
- For radiolabeled DNA, labeling was performed by nick translation. Label the DNA by replacement synthesis with T4 DNA polymerase or label the 5' end with T4 polynucleotide kinase.
- Improper electrophoresis conditions were used. Do not allow voltage to exceed ~20 V/cm. Maintain a temperature <30°C during electrophoresis. Check that the electrophoresis buffer used has sufficient buffering capacity.
- The DNA contained too much salt. Remove excess salt by ethanol precipitation before electrophoresis.
This can happen if the marker was heated. Please ensure that the ladders are not heated before use.
Citations & References (7)
Search citations by name, author, journal title or abstract text
Citations & References
Abstract
A duplex PCR-based assay for measuring the amount of bacterial contamination in a nucleic acid extract from a culture of free-living protists.
Journal:PLoS One
PubMed ID:23593495
'Cultures of heterotrophic protists often require co-culturing with bacteria to act as a source of nutrition. Such cultures will contain varying levels of intrinsic bacterial contamination that can interfere with molecular research and cause problems with the collection of sufficient material for sequencing. Measuring the levels of bacterial contamination for
Identification and characterization of non-saccharomyces spoilage yeasts isolated from Brazilian wines.
Journal:World J Microbiol Biotechnol
PubMed ID:23355138
'The industry of fine wines and also locally consumed table wines is emerging in Brazil with an increasing volume and economic impact. Enologists in this region currently lack information about the prevalence and characteristics of spoilage yeasts, which may contaminate and potentially undervalue Brazilian wines. Herein, we analyzed 50 local
Prostaglandin E2 transactivates EGF receptor: a novel mechanism for promoting colon cancer growth and gastrointestinal hypertrophy.
Journal:Nat Med
PubMed ID:11875501
'Prostaglandins (PGs), bioactive lipid molecules produced by cyclooxygenase enzymes (COX-1 and COX-2), have diverse biological activities, including growth-promoting actions on gastrointestinal mucosa. They are also implicated in the growth of colonic polyps and cancers. However, the precise mechanisms of these trophic actions of PGs remain unclear. As activation of the
Systemically administered gp100 encoding DNA vaccine for melanoma using water-in-oil-in-water multiple emulsion delivery systems.
Journal:
PubMed ID:23702000
'The purpose of this study was to develop a water-in-oil-in-water (W/O/W) multiple emulsions-based vaccine delivery system for plasmid DNA encoding the gp100 peptide antigen for melanoma immunotherapy. The gp100 encoding plasmid DNA was encapsulated in the inner-most aqueous phase of squalane oil containing W/O/W multiple emulsions using a two-step emulsification
Multiplex PCR assay targeting a diguanylate cyclase-encoding gene, cgcA, to differentiate species within the genus Cronobacter.
Journal:Appl Environ Microbiol
PubMed ID:23144142
In a comparison to the widely used Cronobacter rpoB PCR assay, a highly specific multiplexed PCR assay based on cgcA, a diguanylate cyclase gene, that identified all of the targeted six species among 305 Cronobacter isolates was designed. This assay will be a valuable tool for identifying suspected Cronobacter isolates
7 total citations