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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
Unpaired Two Tailed Student’s Ttests, One Way Or Two Way Anova, Followed By Tukey’s Or Sidak’s Post Hoc Test, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
Unpaired Or Paired Two Tailed Student’s T Tests Or Two Way Anova, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 <t>mice/group.</t> <t>Unpaired</t> t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way <t>ANOVA.</t> Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.
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Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 mice/group. Unpaired t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way ANOVA. Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.

Journal: Molecular neurobiology

Article Title: Intracerebral expression of AAV-APOE4 is not sufficient to alter tau burden in two distinct models of tauopathy

doi: 10.1007/s12035-019-01859-4

Figure Lengend Snippet: Neonatal PS19 mice were injected with AAV-APOE4 or AAV-EGFP and aged to 3 months of age. APOE4 expression does not alter human tau transgene, as shown by CP27-immunoreactive total human tau (A). Quantification of tau protein band normalized to GAPDH loading control is shown (B). n=5 mice/group. Unpaired t test. Representative images of CP13 immunoreactivity from 3 month old mice are shown from different regions of the cortex and hippocampal CA1 (C). Scale bar: 100 μm. Quantitation of the immunostaining is presented as % immunoreactivity in the cortex and hippocampus (D). n= 5–11 mice/group. Two way ANOVA. Western blotting with PBS extracted brain lysate (denoted as S1) was done using ptau antibody (CP13, E-F) and total mouse tau antibody (T49, G-H) with protein band normalized to Gapdh loading control (F, H). n=5 mice/group. Unpaired t test. Pretangle tau levels were assessed by MC1 immunostaining in different areas of the cortex and hippocampus CA1 area (I) and data quantified as % immunoreactivity (J). Scale bar: 100 μm. n=5–11 mice/group. Two way ANOVA. Sarkosyl-insoluble cellular fraction (denoted as S4) was assessed for the presence of total human tau (K-L) and total mouse tau (M). n=5 mice/group. Unpaired t test. Black symbols, male mice; grey symbols, female mice.

Article Snippet: Statistical comparisons were conducted using unpaired t tests or 2 Way ANOVA with a Sidak post hoc test, if necessary (GraphPad Prism 7).

Techniques: Injection, Expressing, Control, Quantitation Assay, Immunostaining, Western Blot

Morphometric analysis of the forebrain was done by counting hippocampal CA1–3 neurons and by measuring cortical thickness (frontal cortex, motor/sensory cortex, and auditory cortex) from specific brain areas of 4 month old rTg4510 mice (A-C) or 6 month old rTg4510 mice (J-L). This specific area was bounded by Bregma coordinates: 0.84mm and 1.08mm. Scale bar: 300 μm (larger panels on the left); 125μm (smaller panels on the right). n=4–6 mice/group. Unpaired t test of 2 way ANOVA. Synaptic protein profile was analyzed by immunoblotting for synaptogyrin 3, synaptophysin, spinophilin, PSD95, vGlut1 and GluR1 in the 4 month rTg4510 mice (D-I) and in the 6 month rTg4510 mice (M-R). Indicated protein bands were quantified following normalization to either GAPDH or Actin as shown. n=6/group (4 month rTg4510) and n=4 (6 month rTg4510). Black symbols, male mice; grey symbols, female mice.

Journal: Molecular neurobiology

Article Title: Intracerebral expression of AAV-APOE4 is not sufficient to alter tau burden in two distinct models of tauopathy

doi: 10.1007/s12035-019-01859-4

Figure Lengend Snippet: Morphometric analysis of the forebrain was done by counting hippocampal CA1–3 neurons and by measuring cortical thickness (frontal cortex, motor/sensory cortex, and auditory cortex) from specific brain areas of 4 month old rTg4510 mice (A-C) or 6 month old rTg4510 mice (J-L). This specific area was bounded by Bregma coordinates: 0.84mm and 1.08mm. Scale bar: 300 μm (larger panels on the left); 125μm (smaller panels on the right). n=4–6 mice/group. Unpaired t test of 2 way ANOVA. Synaptic protein profile was analyzed by immunoblotting for synaptogyrin 3, synaptophysin, spinophilin, PSD95, vGlut1 and GluR1 in the 4 month rTg4510 mice (D-I) and in the 6 month rTg4510 mice (M-R). Indicated protein bands were quantified following normalization to either GAPDH or Actin as shown. n=6/group (4 month rTg4510) and n=4 (6 month rTg4510). Black symbols, male mice; grey symbols, female mice.

Article Snippet: Statistical comparisons were conducted using unpaired t tests or 2 Way ANOVA with a Sidak post hoc test, if necessary (GraphPad Prism 7).

Techniques: Western Blot