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Image Search Results
Journal: The Journal of Clinical Endocrinology and Metabolism
Article Title: α-Klotho Expression in Human Tissues
doi: 10.1210/jc.2015-1800
Figure Lengend Snippet: α-Klotho isoforms, sequence, and Western blot. A, Structure of the two isoforms of α-Klotho. Isoform 1 represents the full-length protein and contains a signal sequence domain (SS), two homologous domains (KL1, KL2), a short transmembrane domain (TM), and a short cytoplasmic tail. Shown is the site of the epitope for the antibody used in our experiments: AA 800 to 900, KL2. This epitope is absent from Isoform 2, a soluble, secreted protein that arises from alternative RNA splicing and contains only AA 1–549, and where the terminal 15 residues are replaced by the sequence shown. B, The full-length α-Klotho protein sequence of 1012 AA is shown, with KL1 and KL2 shown in red and green respectively, and TM highlighted (black). The peptides giving rise to the PRM signature are also shown (bold typeface; common to isoforms 1 and 2, red; exclusive to full-length α-Klotho, isoform 1, blue). C and D, Western blot analysis of cell lysates (C) and tissues (D) supports the presence of the full-length α-Klotho. Full-length rh α-Klotho protein (rh-α-Klotho). EC, epithelial cells.
Article Snippet: Cell lysates were obtained from commercially available primary cell cultures (
Techniques: Sequencing, Western Blot
Journal: The Journal of Clinical Endocrinology and Metabolism
Article Title: α-Klotho Expression in Human Tissues
doi: 10.1210/jc.2015-1800
Figure Lengend Snippet: α-Klotho protein expression and distribution in human epithelial and reproductive tissues. IHC, positive staining (brown) was found in all the cellular layers of the epidermis (A) and appendage tissue such as hair follicle and sebaceous gland (B). Intestinal expression was primarily found in epithelial cells as illustrated in jejunum (C) and colon (D). In reproductive tissues, positive staining was found in epithelial Sertoli cells (E), testosterone producing Leydig cells (illustrated with white arrows) of the testis (F), and epithelial cells of the prostate gland G). H–K, In mammary tissue (H), endometrium of uterus (I), and endometrium of salpinx (K), the epithelial cell layer was staining strongly for α-Klotho protein; insets are larger magnifications of the epithelial layer. n ≥ 5 for each tissue.
Article Snippet: Cell lysates were obtained from commercially available primary cell cultures (
Techniques: Expressing, Staining
Journal: The Journal of Clinical Endocrinology and Metabolism
Article Title: α-Klotho Expression in Human Tissues
doi: 10.1210/jc.2015-1800
Figure Lengend Snippet: Mass spectrometry characterization of the transmembrane α-Klotho protein in human tissues and cells: extracellular α-Klotho peptide GLFYVDFLSQKD (exon 3). A–D, Representative mass spectrometry spectra (left) and Skyline data (right) confirmed the presence of full-length α-Klotho rh full-length α-Klotho protein (rh-α-Klotho) (A), renal proximal tubular epithelial cells (B), kidney tissue (C), and renal artery (D). E–G, The full-length specific (isoform 1) αKlotho peptide LWITMNEPYTR (exon 4). Representative mass spectrometry spectra (left) and Skyline data (right) confirmed the presence of full-length α-Klotho. E), rh full-length α-Klotho protein (rh-α-Klotho); F, kidney tissue; G, renal artery; and H, neuronal cells.
Article Snippet: Cell lysates were obtained from commercially available primary cell cultures (
Techniques: Mass Spectrometry, Targeted Proteomics
Journal: The Journal of Clinical Endocrinology and Metabolism
Article Title: α-Klotho Expression in Human Tissues
doi: 10.1210/jc.2015-1800
Figure Lengend Snippet: Confirmation of Transmembrane α-Klotho Protein Expression in Human Tissues and Cells
Article Snippet: Cell lysates were obtained from commercially available primary cell cultures (
Techniques: Expressing, Recombinant
Journal: Cell Death & Disease
Article Title: Cellular senescence promotes macrophage-to-myofibroblast transition in chronic ischemic renal disease
doi: 10.1038/s41419-025-07666-1
Figure Lengend Snippet: SA-β-gal staining ( A ) and the mRNA expression of senescence markers (PAI-1, p16 INK-4a , p21 Cip1/Waf1 , p53, IL-6, MCP-1, TNF-α) ( B – H ) were significantly increased in human renal proximal tubular epithelial cells (HRPTEpiC) following TNF-α and TGF-β treatment. Similarly, the protein levels of IFITM3 were elevated under the same conditions ( I , J ). Data are mean ± SD ( n = 3/group). * P < 0.05 vs. Normal. PAI-1: plasminogen activator inhibitor-1. Scale bar: 200 µm ( A ).
Article Snippet: Firstly,
Techniques: Staining, Expressing
Journal: Cell Death & Disease
Article Title: Cellular senescence promotes macrophage-to-myofibroblast transition in chronic ischemic renal disease
doi: 10.1038/s41419-025-07666-1
Figure Lengend Snippet: A Schematic of the in vitro experimental protocol. B , C : Immunofluorescence staining of Ki67 and quantitative analysis of Ki67 + cells. The number of Ki67 + cells decreased after co-culture with senescent human renal proximal tubular epithelial cells (HRPTEpiC) (senescent cells, SC). Scale bar: 100 µm ( B ). The data are mean ± SD (n = 3/group). D – H : The effects of IFITM-3 and ITGB-3 on macrophage senescence. IFITM3 and ITGB3 were manipulated in SC HRPTEpiC and macrophages, respectively. Macrophages were subsequently collected for Western blot analysis of senescence markers p21 Cip1/Waf1 , p53, p-p53.S15, and γ-H2AX. Silencing ITGB3 or IFITM3 individually using siRNA reduced the expression of these senescence markers. However, this blunting effect was mitigated when IFITM3 was overexpressed in HRPTEpiC, indicating that IFITM3 plays a critical role in maintaining senescence signaling despite ITGB3 knockdown. Data are mean ± SD ( n = 3/group). * P < 0.05 vs. Normal control (NC) and Non-SC groups; # P < 0.05 vs. SC group; and P < 0.05 vs. SC + IFITM3 over-expressing groups. I – K : Relative mRNA expression of the senescence markers p16 INK-4a , p21 Cip1/Waf1 , and p53 increased in macrophages co-incubated with senescent cells. β-actin was used as loading control. Data are mean ± SD ( n = 3/group). * P < 0.05 vs. Normal.
Article Snippet: Firstly,
Techniques: In Vitro, Immunofluorescence, Staining, Co-Culture Assay, Western Blot, Expressing, Knockdown, Control, Incubation
Journal: Nephrology Dialysis Transplantation
Article Title: CRIM1 is localized to the podocyte filtration slit diaphragm of the adult human kidney
doi: 10.1093/ndt/gfn743
Figure Lengend Snippet: Results from real-time quantitative RT-PCR assessment of CRIM1 mRNA levels in two separate cultures of conditionally immortalized podocytes (Podocytes 1 and 2), normal human kidney samples (Normal 1 and 2), primary human renal proximal tubule cells (RPTEC 1 and 2) and primary human pulmonary artery smooth muscle cells (HPASMC 1 and 2). Results are in arbitrary units ± SD. The levels were normalized to three separate housekeeping genes and the identity of the PCR product was confirmed by sequencing.
Article Snippet:
Techniques: Quantitative RT-PCR, Sequencing