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RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in <t>soluble</t> and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.
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RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in <t>soluble</t> and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.
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soluble protein tp  (Nanjing Jiancheng Bioengineering Research Institute Co Ltd)
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RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in <t>soluble</t> and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.
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RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in <t>soluble</t> and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.
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RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in <t>soluble</t> and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.
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Schematic of the Kuppfer cell (KC)-hepatocyte crosstalk mechanism in RILD. Irradiation (IR) stimulates KCs to secrete IL-6, which binds to the <t>IL-6R/gp130</t> complex on hepatocytes to activate JAK; phosphorylated JAK induces STAT3 phosphorylation, and nuclear-translocated p-STAT3 binds to the Ccng1 promoter to promote its transcription; CCNG1 then regulates MDM2 to mediate ubiquitination-dependent TP53 proteolysis, ultimately enhancing hepatocyte apoptosis and driving radiation-induced liver disease (RILD) progression.
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Schematic of the Kuppfer cell (KC)-hepatocyte crosstalk mechanism in RILD. Irradiation (IR) stimulates KCs to secrete IL-6, which binds to the <t>IL-6R/gp130</t> complex on hepatocytes to activate JAK; phosphorylated JAK induces STAT3 phosphorylation, and nuclear-translocated p-STAT3 binds to the Ccng1 promoter to promote its transcription; CCNG1 then regulates MDM2 to mediate ubiquitination-dependent TP53 proteolysis, ultimately enhancing hepatocyte apoptosis and driving radiation-induced liver disease (RILD) progression.
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Image Search Results


RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in soluble and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.

Journal: Journal of Advanced Research

Article Title: Spike RBD drives sustained Parkinson’s disease progression via microglia-neuron crosstalk-mediated RTP801 upregulation

doi: 10.1016/j.jare.2025.07.060

Figure Lengend Snippet: RBD exacerbates degeneration of dopaminergic neurons and αSyn aggregation. (A) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to CSGS 1w + Vehicle group), scale bar = 500 μm, n = 4. (B) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (C) Representative image of Lewy bodies of SNc and quantitative analysis of LB signal intensity (n = 4), scale bar = 50 μm. (D-E) Colocalization of p-αSyn with αSyn in the SNc, quantitative analysis of p-αSyn signal intensity (n = 4), scale bar = 5 μm. (F-G) Colocalization of n-αSyn with αSyn in the SNc, quantitative analysis of n-αSyn signal intensity (n = 4), scale bar = 5 μm. (H) ThS staining quantifies aggregates in the SNc, including ThS signal density and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (I) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( J ) Analysis of αSyn partitioning in soluble and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.

Article Snippet: Soluble and insoluble protein fractions were isolated using a commercially accessible Soluble & Insoluble Protein Extraction Kit (Sangon Biotech, Shanghai, China).

Techniques: Immunostaining, Western Blot, Expressing, Staining

RTP801 is critical for PD deterioration induced by RBD. (A) Schematic of the αSyn A53T + ; RTP801 −/− mice experiment. (B) Assessment of olfactory dysfunction was conducted using the BFPT and the visible BFPT. (C) A modified open field test with nuts or paprika quantified olfactory acuity. (D-F) Motor coordination and balance were evaluated using the rotarod (D) , pole (E) , and beam walking (F) tests. ( G ) Forelimb grip strength was gauged through the grip strength test. ( H ) The open field test appraised anxiety-related behaviors, tracking total distance traveled, center zone activity. (I-J) Recognition memory was assessed using Y maze test and NORT. Alternation index (% of total triplet arm entries) was quantified in (I) . New object index was quantified in ( J ) (n = 6). (K) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to αSyn A53T group), scale bar = 500 μm, n = 4. (L) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (M) Colocalization of RTP801 with TH, scale bar = 200 μm. (N) ThS staining quantifies aggregates in the SNc, including ThS signal density, and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (O) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( P ) Analysis of αSyn partitioning in soluble and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.

Journal: Journal of Advanced Research

Article Title: Spike RBD drives sustained Parkinson’s disease progression via microglia-neuron crosstalk-mediated RTP801 upregulation

doi: 10.1016/j.jare.2025.07.060

Figure Lengend Snippet: RTP801 is critical for PD deterioration induced by RBD. (A) Schematic of the αSyn A53T + ; RTP801 −/− mice experiment. (B) Assessment of olfactory dysfunction was conducted using the BFPT and the visible BFPT. (C) A modified open field test with nuts or paprika quantified olfactory acuity. (D-F) Motor coordination and balance were evaluated using the rotarod (D) , pole (E) , and beam walking (F) tests. ( G ) Forelimb grip strength was gauged through the grip strength test. ( H ) The open field test appraised anxiety-related behaviors, tracking total distance traveled, center zone activity. (I-J) Recognition memory was assessed using Y maze test and NORT. Alternation index (% of total triplet arm entries) was quantified in (I) . New object index was quantified in ( J ) (n = 6). (K) Representative images of TH immunostaining in the SNc and striatum and quantitative assessment (all values were normalized relative to αSyn A53T group), scale bar = 500 μm, n = 4. (L) Western blot analysis of TH expression in SNc and striatum and quantitative analysis (n = 4). (M) Colocalization of RTP801 with TH, scale bar = 200 μm. (N) ThS staining quantifies aggregates in the SNc, including ThS signal density, and the proportion of cells inclusive ThS + puncta (n = 4), scale bar = 5 μm. (O) Western blot detection of αSyn aggregation using the 5G4 antibody, with quantitative analysis confirming significant changes (n = 4). ( P ) Analysis of αSyn partitioning in soluble and insoluble brain fractions by western blot, with quantitative data indicating significant alterations (n = 4). Data are expressed as means ± SEM, * P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant.

Article Snippet: Soluble and insoluble protein fractions were isolated using a commercially accessible Soluble & Insoluble Protein Extraction Kit (Sangon Biotech, Shanghai, China).

Techniques: Olfactory, Modification, Activity Assay, Immunostaining, Western Blot, Expressing, Staining

Schematic of the Kuppfer cell (KC)-hepatocyte crosstalk mechanism in RILD. Irradiation (IR) stimulates KCs to secrete IL-6, which binds to the IL-6R/gp130 complex on hepatocytes to activate JAK; phosphorylated JAK induces STAT3 phosphorylation, and nuclear-translocated p-STAT3 binds to the Ccng1 promoter to promote its transcription; CCNG1 then regulates MDM2 to mediate ubiquitination-dependent TP53 proteolysis, ultimately enhancing hepatocyte apoptosis and driving radiation-induced liver disease (RILD) progression.

Journal: Advances in Radiation Oncology

Article Title: Kupffer Cell-Derived Interleukin-6 Aggravates Radiation-Induced Liver Disease by Activating Hepatocyte STAT3 to Promote Ccng1 Transcription

doi: 10.1016/j.adro.2026.102003

Figure Lengend Snippet: Schematic of the Kuppfer cell (KC)-hepatocyte crosstalk mechanism in RILD. Irradiation (IR) stimulates KCs to secrete IL-6, which binds to the IL-6R/gp130 complex on hepatocytes to activate JAK; phosphorylated JAK induces STAT3 phosphorylation, and nuclear-translocated p-STAT3 binds to the Ccng1 promoter to promote its transcription; CCNG1 then regulates MDM2 to mediate ubiquitination-dependent TP53 proteolysis, ultimately enhancing hepatocyte apoptosis and driving radiation-induced liver disease (RILD) progression.

Article Snippet: Either a rat interleukin (IL)-6 antibody (anti-IL-6; R&D Systems, #AF506) or soluble rat gp130 Fc chimera protein (sgp130Fc; R&D Systems, #5029-RG-100) was intraperitoneally injected twice weekly at concentrations of 16.7 μg/kg and 0.5 mg/kg, respectively.

Techniques: Irradiation, Phospho-proteomics, Ubiquitin Proteomics