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PerCP Conjugated to Secondary Antibodies |
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Nuovo fluorocromo PerCP per la coniugazione di anticorpi secondari dalla Jackson ImmunoResearch
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GAMMA COMPLETA ANTICORPI SECONDARI Clicca qui
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| PerCP is a fluorescent peridinin-chlorophyll protein complex isolated from dinoflagellates. We offer the form found in Dinophyceae
sp. with a molecular weight of about 35.5 kDa. It has a broad spectrum
of excitation with a main peak at 472 nm, and a long Stokes shift to an
emission peak at 677 nm (Figure 1). |
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| Figure 1. Relative shape and position of spectra in the peak region of
excitation (blue) and emission (purple) for PerCP conjugated to an
affinity-purified secondary antibody from Jackson ImmunoResearch.
Quantitative comparisons should not be made since peak heights have
been normalized. Spectra were obtained with an M-Series
spectrofluorometer system from Photon Technology International, Inc. |
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| PerCP conjugates of highly adsorbed secondary
antibodies are offered to label unconjugated primary antibodies, and
PerCP-streptavidin is offered to label biotinylated primary or
secondary antibodies (Figures 2 and 3). Two practical labeling
protocols are possible with these products. Compared with a single-step
PerCP-conjugated primary antibody (Figure 2), about the same level of
fluorescence is obtained with a two-step procedure using a biotinylated
primary antibody and PerCP-conjugated streptavidin. A consistent,
slightly higher signal is achieved by using an unconjugated primary
antibody and PerCP-conjugated secondary antibody. Although three-step
procedures are usually undesirable for flow cytometry, a somewhat
greater amplification may be obtained with unconjugated primary
antibody, biotinylated secondary antibody, and PerCP-conjugated
streptavidin (Figure 3). |
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| Figure 2. Human peripheral lymphocytes were stained either directly
with PerCP-conjugated anti-CD3 (orange) from BioLegend, or indirectly
with biotin-conjugated anti-CD3 (B-D Pharmingen) and PerCP-streptavidin
either from Jackson ImmunoResearch (blue), BioLegend (purple), or B-D
Pharmingen (red). For further comparison, cells were stained with
unconjugated anti-CD3 (B-D Pharmingen) and PerCP-conjugated secondary
antibody from Jackson Immuno-Research (green). Stained cells were
analyzed in a dual-laser FACSCalibur flow cytometer (Becton Dickinson).
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Figure
3. Human peripheral lymphocytes were stained with unconjugated anti-CD3
(B-D Pharmingen) and PerCP-conju-gated secondary antibody from Jackson
ImmunoResearch (green), or with biotin-conjugated anti-CD3 (B-D
Pharmingen) and PerCP-streptavidin from Jackson ImmunoResearch (blue).
For further comparison, cells were stained with unconjugated anti-CD3
(B-D Pharmingen), biotinylated secondary antibody and
PerCP-streptavidin from Jackson ImmunoResearch (red). Stained cells
were analyzed in a dual-laser FACSCalibur flow cytometer (Becton
Dickinson) |
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| PerCP conjugates may be used alone or with DyLight 488 (or FITC) and
R-PE for one- to three-color analyses with a single-laser flow
cytometer equipped with an argon laser emiting at 488 nm. Up to
four-color analyses with low compensation are easily achieved by adding
APC-conjugated antibodies with 633 or 635 nm excitation provided by a
dual-laser flow cytometer (Figure 4). |
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| Figure 4. Excitation spectra (left) for PerCP-(blue), DyLight 488/FITC-
(green), R-PE- (red), and APC- (brown) conjugated secondary antibodies
from Jackson ImmunoResearch. Emission spectra (right) for DyLight
488/FITC- (green), R-PE- (pink), APC- (brown), and PerCP- (purple)
conjugated secondary antibodies from Jackson ImmunoResearch.
Quantitative comparisons should not be made since peak heights have
been normalized. All spectra were obtained with an M-Series
spectrofluorometer system from Photon Technology International, Inc. |
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| See Table of NEW PerCP Conjugates here |
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Per ulteriori informazioni CONTATTACI
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