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43069

Atto 565 azide

Name: Atto 565 azide
Brand: SIGMA

BioReagent, suitable for fluorescence, ≥80.0% (HPCE)

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About This Item

UNSPSC Code:

12352200

NACRES:

NA.32

product line

BioReagent

assay

≥80.0% (HPCE)

manufacturer/tradename

ATTO-TEC GmbH

fluorescence

λ_ex 565 nm; λ_em 592 nm±10 nm in 0.1 M phosphate pH 7.0

suitability

suitable for fluorescence

storage temp.

−20°C

Legal Information

This product is for Research use only. In case of intended commercialization, please contact the IP-holder (ATTO-TEC GmbH, Germany) for licensing.

Storage Class

11 - Combustible Solids

wgk_germany

WGK 3

flash_point_f

Not applicable

flash_point_c

Not applicable

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Lot/Batch Number

BCBP4898V

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Specific and stable fluorescence labeling of histidine-tagged proteins for dissecting multi-protein complex formation.

Suman Lata et al.

Journal of the American Chemical Society, 128(7), 2365-2372 (2006-02-16)

Labeling of proteins with fluorescent dyes offers powerful means for monitoring protein interactions in vitro and in live cells. Only a few techniques for noncovalent fluorescence labeling with well-defined localization of the attached dye are currently available. Here, we present

Preferential binding of a kinesin-1 motor to GTP-tubulin-rich microtubules underlies polarized vesicle transport.

Takao Nakata et al.

The Journal of cell biology, 194(2), 245-255 (2011-07-20)

Polarized transport in neurons is fundamental for the formation of neuronal circuitry. A motor domain-containing truncated KIF5 (a kinesin-1) recognizes axonal microtubules, which are enriched in EB1 binding sites, and selectively accumulates at the tips of axons. However, it remains

Spectroelectrochemical investigation of intramolecular and interfacial electron-transfer rates reveals differences between nitrite reductase at rest and during turnover.

Łukasz Krzemiński et al.

Journal of the American Chemical Society, 133(38), 15085-15093 (2011-08-26)

A combined fluorescence and electrochemical method is described that is used to simultaneously monitor the type-1 copper oxidation state and the nitrite turnover rate of a nitrite reductase (NiR) from Alcaligenes faecalis S-6. The catalytic activity of NiR is measured

Complementary methods provide evidence for the expression of CXCR7 on human B cells.

Marie-Luise Humpert et al.

Proteomics, 12(12), 1938-1948 (2012-05-25)

PTMs of extracellular domains of membrane proteins can influence antibody binding and give rise to ambivalent results. Best proof of protein expression is the use of complementary methods to provide unequivocal evidence. CXCR7, a member of the atypical chemokine receptor

PALM and STORM. Unlocking live-cell super-resolution.

Henriques, R.; Griffiths, C.; Hesper Rego, E.; Mhlanga, Musa M.

Biopolymers, 95(5), 322-331 (2011)

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