Anti hq hrp

Manufactured by Roche

The Anti-HQ HRP is a laboratory reagent used to detect and quantify the presence of a specific target analyte. It contains an antibody conjugated to the horseradish peroxidase (HRP) enzyme, which serves as a label for the detection process. The core function of this product is to provide a sensitive and reliable method for the immunoassay-based identification and measurement of the target analyte in various sample types.

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Lab products found in correlation

Anti rabbit hq, by Roche (3 mentions) Cell conditioning 1 cc1, by Roche (3 mentions) Hematoxylin and bluing reagent, by Roche (2 mentions) Discovery chromomap dab kit, by Roche (1 mentions) Scn400 slide scanner, by Leica Microsystems (1 mentions) Discovery ultra, by Roche (1 mentions) Aperio imagescope, by Leica Biosystems (1 mentions) Ez prep solution, by Roche (1 mentions) Chromomap dab detection kit, by Roche (1 mentions) Optiview dab detection kit, by Roche (1 mentions) Anti mouse hq, by Roche (1 mentions) Ventana benchmark discovery, by Roche (1 mentions) Mrq 42, by Cell Marque (1 mentions)

4 protocols using anti hq hrp

Automated Immunohistochemistry Staining for Abi1

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Immunohistochemistry was performed on TMA sections with the automated immunohistochemistry staining platform DISCOVERY ULTRA (Ventana Medical Systems, Inc.). Antigen retrieval was conducted with Cell Conditioning 1 (CC1) (Ventana) at 95 °C for 64 min. Slides were incubated with a 1:200 dilution of Abi1 antibody (Cell Signaling Technologies, 39444S) at room temperature for 2 h. For detection, a DISCOVERY ChromoMap DAB Kit, anti-HQ HRP, and anti-rabbit HQ (Ventana) were used. Digital images of stained TMAs were acquired with an SCN400 Slide Scanner (Leica Microsystems). Positively stained cells were analyzed with Aperio ImageScope (Leica Biosystems).

Nath D., Li X., Mondragon C., Post D., Chen M., White J.R., Hryniewicz-Jankowska A., Caza T., Kuznetsov V.A., Hehnly H., Jamaspishvili T., Berman D.M., Zhang F., Kung S.H., Fazli L., Gleave M.E., Bratslavsky G., Pandolfi P.P, & Kotula L. (2019). Abi1 loss drives prostate tumorigenesis through activation of EMT and non-canonical WNT signaling. Cell Communication and Signaling : CCS, 17, 120.

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Immunohistochemical Profiling of FFPE Tumor Samples

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Immunohistochemistry of the FFPE tumor samples was performed on a BenchMark Ultra autostainer (TLE3) or Discovery Ultra autostainer (Glucocorticoid Receptor). Briefly, paraffin sections were cut at 3 µm, heated at 75°C for 28 min and deparaffinized in the instrument with EZ prep solution (Ventana Medical Systems). Heat-induced antigen retrieval was carried out using Cell Conditioning 1 (CC1, Ventana Medical Systems) for 64 min at 95°C.Glucocorticoid Receptor clone D6H2L (Cell Signaling) was detected using 1/600 dilution, 1 hr at 37⁰C and TLE3 using clone CL3573 (1/250 dilution, 1 hr at RT). Bound TLE3 was detected using the OptiView DAB Detection Kit (Ventana Medical Systems). Glucocorticoid Receptor bound antibody was visualized using Anti-Rabbit HQ (Ventana Medical systems) for 12 min at 37⁰C, Anti-HQ HRP (Ventana Medical systems) for 12 min at 37°C, followed by ChromoMap DAB Detection Kit (Ventana Medical Systems). Slides were counterstained with Hematoxylin and Bluing Reagent (Ventana Medical Systems).

Palit S.A., Vis D., Stelloo S., Lieftink C., Prekovic S., Bekers E., Hofland I., Šuštić T., Wolters L., Beijersbergen R., Bergman A.M., Győrffy B., Wessels L.F., Zwart W, & van der Heijden M.S. (2019). TLE3 loss confers AR inhibitor resistance by facilitating GR-mediated human prostate cancer cell growth. eLife, 8, e47430.

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Immunostaining Protocol for M1/M2 Macrophages

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Sections of 4µm of FFPE samples were used for immunohistochemistry analysis. To visualize M1 and M2 macrophage subsets in placental tissue, the chromogenic duplex staining was done with CD68 and CD163 by an automated staining procedure using the Ventana Benchmark Discovery (Ventana Medical Systems Inc.). In brief, following deparaffinization and heat-induced antigen retrieval with CC1 (#950-500, Ventana) for 40 minutes at 95°C, the tissue samples were firstly incubated with CD68 for 60 minutes at 37˚C, followed by detection with anti-mouse HQ (#760-4814, Ventana) for 16 minutes and subsequently anti-HQ HRP (#760-4820), and visualized with Discovery Purple (#760-229, Ventana) for 32 minutes. An antibody denature step was performed using CC2 (#950-123, Ventana) for 20 minutes at 100˚C. Secondly, CD163 was incubated for 32 minutes at 37˚C, followed by detection with anti-mouse HQ and subsequently anti-HQ HRP, and visualized with Discovery Teal (#760-247, Ventana) for 32 minutes. Finally, all slides were counterstained with hematoxylin II (#760-2208) and bluing reagents (#760-2037) for 4 minutes. Antibody information and clonality can be found in Supplementary Table S3.

Broekhuizen M., Hitzerd E., van den Bosch T.P., Dumas J., Verdijk R.M., van Rijn B.B., Danser A.H., van Eijck C.H., Reiss I.K, & Mustafa D.A. (2021). The Placental Innate Immune System Is Altered in Early-Onset Preeclampsia, but Not in Late-Onset Preeclampsia. Frontiers in Immunology, 12, 780043.

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Multiplex Immunohistochemistry for Immune Profiling

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Details on mutational analysis and immunohistochemical (IHC) staining for PD-L1 expression and CD8 infiltration was previously reported [9 (link)]. Double staining CD3 (yellow) followed by CD56 (purple) of whole slide sections prepared from FFPE resection specimens was performed on a Discovery Ultra autostainer. Slides were deparaffinised in the instrument and heat-induced antigen retrieval was carried out using Cell Conditioning 1 (CC1, Ventana Medical Systems) for 32 min at 95 °C. The CD3 was detected in the first sequence using clone SP7 (1/100 dilution, 32 min at 37 °C, ThermoScientific). CD3 bound antibody was visualized using Anti-Rabbit NP (Ventana Medical systems) for 12 min at 37 °C followed by Anti-NP AP (Ventana Medical systems) for 12 min at 37 °C, followed by the Discovery Yellow detection kit (Ventana Medical Systems). In the second sequence of the double staining procedure CD56 was detected using clone MRQ-42 (1:2000 dilution, 32 min at 37 °C, Cell Marque). CD56 was visualized using Anti-Rabbit HQ (Ventana Medical systems) for 12 min at 37 °C followed by Anti-HQ HRP (Ventana Medical systems) for 12 min at 37 °C, followed by the Discovery Purple Detection Kit (Ventana Medical Systems). Slides were counterstained with Hematoxylin and Bluing Reagent (Ventana Medical Systems).

Theelen W.S., Krijgsman O., Monkhorst K., Kuilman T., Peters D.D., Cornelissen S., Ligtenberg M.A., Willems S.M., Blaauwgeers J.L., van Noesel C.J., Peeper D.S., van den Heuvel M.M, & Schulze K. (2020). Presence of a 34-gene signature is a favorable prognostic marker in squamous non-small cell lung carcinoma. Journal of Translational Medicine, 18, 271.

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