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Df1485

Manufactured by Leica
Sourced in United Kingdom

The DF1485 is a high-precision optical density filter from Leica. It is designed to provide accurate and consistent optical density measurements in laboratory settings. The product specifications and technical details are available upon request.

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2 protocols using df1485

1

Immunohistochemical Profiling of Breast Tumors

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Tumor samples were distributed in 15 TMAs using 4 mm tissue cores at the Experimental Pathology Laboratory of Pontifical Catholic University of Paraná (PUCPR). From each donor block was extracted one or two cylinders 4 mm in diameter and deposited in the receiver blocks, previously prepared. In each TMA, a sample of normal breast tissue was included as an internal control. Thereafter, 4 μm tissue sections from the TMA blocks were transferred to electrically charged Star Frost® (Braunschweig, Germany) slides and incubated with primary antibodies [anti-CD44 (anti-human mouse monoclonal, clone DF1485, dilution 1/40, Novocastra, Newcastle, UK), anti-CD44v6 (antihuman mouse monoclonal, clone VFF-7, dilution 1/100, Novocastra, Newcastle, UK), anti-CD24 (anti-human rabbit polyclonal, dilution 1/200, Abbiotec, San Diego, CA, USA), and anti-ALDH1 (anti-human rabbit monoclonal, clone E-P1932y, dilution 1/100, Epitomics, Cambridge, Massachusetts, USA)] for 12 h in a humidified chamber at 2−8°C. An Advance Dako (Caripenteria, CA, USA) secondary antibody was incubated with the slides for 30 min at 2−8°C. The reactions were developed using a DAB chromogen-substrate solution (Dako). Harris hematoxylin was used for counterstaining. Positive and negative (incubated without primary antibody) controls were run in parallel with all reactions.
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2

CD44 Expression and Survival Analysis

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The paraffin block sample was examined for CD44 expression using CD44 antibody (DF1485, Novocastra Laboratories Ltd., dilution 1:100) then count the percentage of positive cells and their intensity visually using a comparison light microscope. Immunostained samples were evaluated blind by one pathologist. CD44 was stained in cell membrane, with score 0 if < 10% positive tumour cells; FIGURE 1 shows the OS analysis using median with following up to 3 years for survival that could be divided into two groups. From month 0 to 5 th month, the survival rate for OS with low and high CD44 expressions was similar with OS value of 75%. Decrease in 35% survival rate of patients with high CD44 expression was observed on the 10 th month, where as for patients with low CD44 expression on the 17 th month. Furthermore, the patients with high CD44 expression showed a progressive decrease in survival rate from month to month. In the 20 th month, the survival rate decreased to be <15% and then 0-5% in the 25 th month. The decrease in survival rate of patients with low CD44 expression in the 20 th , 25 th , 30 th , and 40 th moths were 20%, 15-20%, 10% and 5-10%, respectively. No significantly relationship between CD44 expression and OS was observed (p>0.05).
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