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Donkey anti goatalexa488 secondary antibody

Manufactured by Thermo Fisher Scientific
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Donkey anti-goat Alexa488 secondary antibody is a fluorescently labeled antibody used in immunoassays to detect the presence of goat primary antibodies. The Alexa488 fluorophore emits green fluorescence when excited, allowing for visualization and quantification of target proteins or cells.

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Lab products found in correlation

Rnascope multiplex fluorescent v2 assay, by Bio-Techne (2 mentions) Mm ppib c1, by Bio-Techne (2 mentions) Dapb c1, by Bio-Techne (2 mentions) Fluoromountg, by BioConcept (2 mentions) Mm gpbar1 c1, by Bio-Techne (2 mentions) Mm agrp c2, by Bio-Techne (2 mentions) Tsa plus cy3, by PerkinElmer (2 mentions) Withfluoromountg, by BioConcept (2 mentions) Goat anti gfp primary antibody, by Abcam (2 mentions) Lsm 700 confocal microscope, by Zeiss (2 mentions)

3 protocols using donkey anti goatalexa488 secondary antibody

1

Multiplex RNAscope Fluorescent Imaging of Metabolic Genes

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RNAscope Multiplex Fluorescent V2 assay (Bio-techne, Cat#:323110) was
performed according to manufacturer’s instruction on 4 μm paraffin
sections, hybridized with the probes Mm-Gpbar1-C1(Bio-techne, Cat#:318451),
Mm-Agrp-C2 (Bio-techne, Cat#:400711-C2), Mm-Ppib-C1 (Bio-techne, Cat#:313911) as
positive control and DapB-C1 (Bio-techne, Cat#:310043) as negative control at
40°C for 2 hours and revealed with TSA Plus Cy3 (Perkin Elmer,
Cat#:NEL744E001KT). Tissues were counterstained with DAPI and mounted with
FluoromountG (Bioconcept, Cat#:100.01). When indicated, sections were incubated
overnight at 4°C with a goat anti-GFP primary antibody (Abcam,
Cat#:ab6673 – 1:200 dilution). After incubation with a donkey anti-goat
Alexa488 secondary antibody (Thermo Fisher, Cat#:A11055, 1:1000 dilution),
tissues were counterstained with DAPI and mounted with FluoromountG (Bioconcept,
Cat#:100.01). The imaging was performed with Zeiss LSM 700 confocal microscope
(Carl Zeiss Microscopy, Germany).
Perino A., Velázquez-Villegas L.A., Bresciani N., Sun Y., Huang Q., Fénelon V.S., Castellanos-Jankiewicz A., Zizzari P., Bruschetta G., Jin S., Baleisyte A., Gioiello A., Pellicciari R., Ivanisevic J., Schneider B.L., Diano S., Cota D, & Schoonjans K. (2021). Central anorexigenic actions of bile acids are mediated by TGR5. Nature metabolism, 3(5), 595-603.
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2

Multiplex RNAscope Fluorescent Imaging of Metabolic Genes

Check if the same lab product or an alternative is used in the 5 most similar protocols
RNAscope Multiplex Fluorescent V2 assay (Bio-techne, Cat#:323110) was
performed according to manufacturer’s instruction on 4 μm paraffin
sections, hybridized with the probes Mm-Gpbar1-C1(Bio-techne, Cat#:318451),
Mm-Agrp-C2 (Bio-techne, Cat#:400711-C2), Mm-Ppib-C1 (Bio-techne, Cat#:313911) as
positive control and DapB-C1 (Bio-techne, Cat#:310043) as negative control at
40°C for 2 hours and revealed with TSA Plus Cy3 (Perkin Elmer,
Cat#:NEL744E001KT). Tissues were counterstained with DAPI and mounted with
FluoromountG (Bioconcept, Cat#:100.01). When indicated, sections were incubated
overnight at 4°C with a goat anti-GFP primary antibody (Abcam,
Cat#:ab6673 – 1:200 dilution). After incubation with a donkey anti-goat
Alexa488 secondary antibody (Thermo Fisher, Cat#:A11055, 1:1000 dilution),
tissues were counterstained with DAPI and mounted with FluoromountG (Bioconcept,
Cat#:100.01). The imaging was performed with Zeiss LSM 700 confocal microscope
(Carl Zeiss Microscopy, Germany).
Perino A., Velázquez-Villegas L.A., Bresciani N., Sun Y., Huang Q., Fénelon V.S., Castellanos-Jankiewicz A., Zizzari P., Bruschetta G., Jin S., Baleisyte A., Gioiello A., Pellicciari R., Ivanisevic J., Schneider B.L., Diano S., Cota D, & Schoonjans K. (2021). Central anorexigenic actions of bile acids are mediated by TGR5. Nature metabolism, 3(5), 595-603.
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3

Visualizing Viral Protein Localization

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Tomato (Solanum lycopersicum) 'Tamina' plants were grown for 24 days and then Agroinfiltrated. Agrobacteria carried several PVX constructs (PVX-empty vector, PVX-GFP and PVXΔCP-GFP). Small leaf discs were collected at 10 dpi for immune-staining. Segments of leaves were fixed with 3 % para-formaldehyde/0.05 % Triton TM X-100 in PBS for 3 hours at room temperature and subsequently embedded in PEG 1500 as described in (51). GFP was labelled in 3 µm sections with a polyclonal antibody from goat (# 600-101-215; Rockland; diluted 1:500 in PBS containing 5% bovine serum albumin) detected with a donkey-anti-goat-Alexa 488 secondary antibody (# A-11055, Thermo Fisher Scientific; diluted 1:500 in PBS containing 5% bovine serum albumin).
Torti S., Schlesier R., Thümmler A., Bartels D., Römer P., Koch B., Werner S., Panwar V., Kanyuka K., Wirén N.V., Jones J.D.G., Hause G., Giritch A, & Gleba Y. (2021). Transient reprogramming of crop plants for agronomic performance. Nature plants, 7(2).
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