Immediately after samples were removed from culture, they were placed in 4% paraformaldehyde for fixation for at least one week and then embedded in paraffin. Once all samples were in paraffin, they were sectioned along the sagittal plane and stained on the same day. Tissue were stained with hematoxylin and eosin for morphological analysis, α-smooth muscle actin α-SMA (clone 14A, Cell Marque) for myofibroblast formation and intercapsular adhesion28 (link)–30 (link), Ki-67 (clone 30–9, Ventana) for proliferation31 (link) and vimentin (clone V9, Ventana) a marker of both undifferentiated lens epithelium as well as differentiating fiber cells32 (link). All immunostainings were done with the BenchMark® ULTRA device (Ventana Medical Systems, Inc.). We also included negative immunostain controls to support the validity of our stains and identify possible experimental artefacts or background noise. These controls were processed in the same manner with the automated staining device but without the primary antibodies. Capsular adhesion, cellular morphology and the degree of staining of α-SMA, Ki-67 and vimentin were studied at the equatorial region of the capsule and at the center of the posterior capsule.
Vimentin clone v9
Manufactured by Roche
Vimentin (clone V9) is a laboratory reagent used for the detection of vimentin, an intermediate filament protein. Vimentin is a structural protein found in various cell types and is commonly used as a marker in immunohistochemistry and cell biology applications. The clone V9 is a specific antibody that binds to vimentin and can be used to identify and visualize cells expressing this protein.
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Lab products found in correlation
2 protocols using vimentin clone v9
1
Histological Characterization of Lens Capsule
2
Histological Evaluation of Wound Tissue
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The obtained slough was quickly fixed in 10% neutral buffered formalin solution, embedded in paraffin, and cut into 4-μm-thick sections perpendicular to the surface. Hematoxylin/eosin (H/E) staining and Azan–Mallory (A/M) staining were performed. Immunostaining was performed to identify the following cell types: CD33 (clone PWS44, 1×, Leica) for neutrophils, CD68 (clone KP1, 1×, DAKO) for macrophages, CD31 (clone JC70A, 1×, DAKO) for endothelial cells, vimentin (clone V9, 1×, Ventana) for mesenchymal cells, and α-smooth muscle actin (αSMA; clone 1A4, 1×, DAKO) for smooth muscle cells.
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