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Ab54966

Manufactured by Abcam
Sourced in United Kingdom

Ab54966 is a laboratory equipment product manufactured by Abcam. It is a tool used for scientific research and analysis purposes. The core function of this product is to facilitate the measurement and quantification of specific targets or analytes within a sample.

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4 protocols using ab54966

1

Validating PRIM1 Downstream Targets

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To verify the downstream genes regulated by PRIM1, western blot analyses were performed with anti-JUN (Abcam, ab32137), anti-EGR1 (Abcam, ab54966), anti-MET (Abcam, ab51067), anti-Wnt5a (CST, #2392), anti-PPP2R2C (Abcam, ab172086), anti-IRS (abcam, ab52167), and anti-GAPDH (Santa Cruz, SC-32233) antibodies. All experiments were repeated three times.
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2

Immunohistochemical Analysis of Cancer Markers

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Consecutive sections (4-μm) of tissue microarray samples were mounted on the APES-coated slides. After de-paraffinization, rehydration and antigen retrieval using an autoclave-oven-technique, sections were incubated with anti-PRR11 (HPA023923, SIGMA-ALDRICH), UCHL1 (HPA005993, SIGMA-ALDRICH), SNAT1 (ab59721, abcam®), and EGR1 (ab54966, abcam®) at 4°C overnight. A two-step EnVisionTM KIT (DAKO, USA) was used to visualize positive staining. Lung cancers known to be positive for these proteins were used as positive controls. Replacement of the primary antibody by PBS served as a negative control.
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3

Western Blotting Analysis of Cell Lysates

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Whole cell lysates were used for western blotting analysis as previously described [38 (link), 39 (link)], with glyceraldehyde 3-phosphate dehydrogenase (GAPDH) used as a loading control. The anti-CTCF antibody (07–729) was obtained from Millipore, while antibodies against EGR1 (ab54966), TNFAIP3 (ab74037), GADD45A (ab180768), and p65 (ab16502) were obtained from Abcam; a GAPDH monoclonal antibody (SC-32233) and rabbit or mouse secondary antibodies were purchased from Santa Cruz Biotechnology. The anti-phospho-NF-κB p65 (Ser536) (93H1) antibody was obtained from Cell Signaling.
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4

Immunohistochemical Analysis of PRR11, N-cadherin, and EGR1

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TMA sections were processed for immunohistochemistry (IHC) after depara nization and rehydration routine procedures. Antibody antigen retrieval was performed using tissue submersion in citrate buffer (10 mM, pH 6.0) with heating. Sections were then incubated with an anti-PRR11 antibody (HPA023923, Sigma-Aldrich; Saint Louis, MO, US), anti-ki-67 (cat. 27309-1-AP, proteintech; Wuhan, China), anti-Ncadherin (cat. 610920, BD Biosciences; San Jose, CA, US) and anti-early growth response protein 1 [EGR1] (ab54966, Abcam; Cambridge, UK) at 4℃ overnight. Subsequently, a two-step Envision kit (Agilent Technologies; Santa Clara, CA, US) was used to visualize positive staining. PRR11, N-cadherin, and EGR1 protein expression was evaluated by two researchers who were blind to this study using an Olympus CX31 microscope (Olympus Co; Tokyo, Japan). The antibodies were diluted with 1:100 goat serum for IHC analysis. Positivity was calculated by the semiquantitative scoring system described previously [15] . Generally, IHC staining intensity was assigned as: negative, 0; weak, 1; moderate, 2; and intense; 3. The percentage of IHC positive cells was scored as 0 to 1 (0% to100%). Theoretically, a weighted score ranging from 0 (0% of cells staining) to 3 (100% of the cells staining at 3+ intensity) was generated for each tissue core. An IHC score bigger than (>) 0 was considered positive.
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