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rabbit polyclonal anti drd 1 antibody  (Bioss)


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    Bioss rabbit polyclonal anti drd 1 antibody
    Rabbit Polyclonal Anti Drd 1 Antibody, supplied by Bioss, used in various techniques. Bioz Stars score: 94/100, based on 6 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Average 94 stars, based on 6 article reviews
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    <t>D1-like</t> receptor activity promotes the inhibitory effect of DA on cell contraction, whereas D2-like receptor activity, particularly that of DRD2 in the posterior sclera, impedes it. ( a – p ) The cell contraction rates at 24 hours for anterior ( a – h ) and posterior ( i – p ) scleral fibroblasts from HSF12 and HSF13 were measured following treatment with a range of DA receptor antagonists and agonists, administered 1 hour prior to the addition of DA. One experiment was conducted with three replicate wells for each compound tested, using two biological samples (HSF12 and HSF13; total n = 6). Results from the two cell lines were averaged and presented as mean ± SEM. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001 (two-way ANOVA).
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    <t>D1-like</t> receptor activity promotes the inhibitory effect of DA on cell contraction, whereas D2-like receptor activity, particularly that of DRD2 in the posterior sclera, impedes it. ( a – p ) The cell contraction rates at 24 hours for anterior ( a – h ) and posterior ( i – p ) scleral fibroblasts from HSF12 and HSF13 were measured following treatment with a range of DA receptor antagonists and agonists, administered 1 hour prior to the addition of DA. One experiment was conducted with three replicate wells for each compound tested, using two biological samples (HSF12 and HSF13; total n = 6). Results from the two cell lines were averaged and presented as mean ± SEM. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001 (two-way ANOVA).
    Rabbit Polyclonal Anti Drd1 Antibody, supplied by Bioss, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Deregulated hippocampal GHSR and synaptic function in 24-month-old hAβ KI mice. A, B) Hippocampal GHSR level in (A) 14- and (B) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 3 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 200 μm (inset scale = 30 μm). C, D) Hippocampal GHSR/β-arrestin 2 complex level in (C) 14- and (D) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old nonTg n = 3 males, 2 females, hAβ KI n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). E, F) Hippocampal <t>GHSR/DRD1</t> complex level in (E) 14- and (F) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). G, H) Hippocampal CamKII activation in (G) 14- and (H) 24-month-old hAβ KI mice and the nonTg controls represented by CamKII Thr286 phosphorylation. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females; 24-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females. Bottom panels are the representative images, scale bar = 30 μm. I, J) Hippocampal synaptic density in (I) 14- and (J) 24-month-old hAβ KI mice and the nonTg controls represented by the overlap of presynapse marker vGlut1 and postsynapse marker PSD95. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 2 males, 2 females; 24-month-old nonTg n = 2 males, 2 females; hAβ KI n = 2 males, 1 female. Bottom panels are the representative images, scale bar = 100 μm (inset scale = 10 μm). NS = not significant, *p < 0.05. Females: filled circles, males: open circles.
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    Deregulated hippocampal GHSR and synaptic function in 24-month-old hAβ KI mice. A, B) Hippocampal GHSR level in (A) 14- and (B) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 3 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 200 μm (inset scale = 30 μm). C, D) Hippocampal GHSR/β-arrestin 2 complex level in (C) 14- and (D) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old nonTg n = 3 males, 2 females, hAβ KI n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). E, F) Hippocampal <t>GHSR/DRD1</t> complex level in (E) 14- and (F) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). G, H) Hippocampal CamKII activation in (G) 14- and (H) 24-month-old hAβ KI mice and the nonTg controls represented by CamKII Thr286 phosphorylation. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females; 24-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females. Bottom panels are the representative images, scale bar = 30 μm. I, J) Hippocampal synaptic density in (I) 14- and (J) 24-month-old hAβ KI mice and the nonTg controls represented by the overlap of presynapse marker vGlut1 and postsynapse marker PSD95. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 2 males, 2 females; 24-month-old nonTg n = 2 males, 2 females; hAβ KI n = 2 males, 1 female. Bottom panels are the representative images, scale bar = 100 μm (inset scale = 10 μm). NS = not significant, *p < 0.05. Females: filled circles, males: open circles.
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    rabbit polyclonal anti drd1  (Bioss)
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    Western blots. A A typical Western blot for the D 1 receptor in hearts from WT, D 1 -TG, and D 1 -KO after incubation with the D 1 -dopamine receptor antibody is seen. The corresponding band for the D 1 receptor <t>(DRD1)</t> is labelled with an arrow. As loading control, the Ponceau S-stained membrane is shown below. B Typical Western blots for regulatory proteins in hearts from WT and D 1 -TG after incubation with the D 1 -dopamine receptor agonist SKF 38393 are seen. Western blots depict the phosphorylation state of inhibitory subunit of troponin (P-TnI) with arrows. As a loading control, we assessed the protein expression of cardiac calsequestrin (CSQ) by cutting horizontally the lanes of the blot and incubating the lower and upper halves with different primary antibodies. M rainbow marker, LA left atrium, RA right atrium, VT ventricle
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    rabbit polyclonal anti-dopamine receptor d1 (drd1  (Santa Cruz Biotechnology)
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    HF, Hizikia fusiformis extract treatment; VEH, vehicle treatment (control); <t>DRD1-5,</t> dopamine <t>D1–5</t> receptors; DAT, dopamine transporter; DAPI, 4′,6-diamidino-2-phenylindole; NF-L, neurofilament light chain; SERT, serotonin transporter; TH, tyrosine hydroxylase; TPH, tryptophan hydroxylase; SYP, synaptophysin; 5HT1A and 1B, serotonin 1A and 1B receptors; MAP2, microtubule-associated protein 2.
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    Image Search Results


    D1-like receptor activity promotes the inhibitory effect of DA on cell contraction, whereas D2-like receptor activity, particularly that of DRD2 in the posterior sclera, impedes it. ( a – p ) The cell contraction rates at 24 hours for anterior ( a – h ) and posterior ( i – p ) scleral fibroblasts from HSF12 and HSF13 were measured following treatment with a range of DA receptor antagonists and agonists, administered 1 hour prior to the addition of DA. One experiment was conducted with three replicate wells for each compound tested, using two biological samples (HSF12 and HSF13; total n = 6). Results from the two cell lines were averaged and presented as mean ± SEM. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001 (two-way ANOVA).

    Journal: Investigative Ophthalmology & Visual Science

    Article Title: Distinct Transcriptomic Profiles of Cultured Anterior and Posterior Populations of Human Infant Scleral Fibroblasts: Including Dopamine Receptors

    doi: 10.1167/iovs.66.5.29

    Figure Lengend Snippet: D1-like receptor activity promotes the inhibitory effect of DA on cell contraction, whereas D2-like receptor activity, particularly that of DRD2 in the posterior sclera, impedes it. ( a – p ) The cell contraction rates at 24 hours for anterior ( a – h ) and posterior ( i – p ) scleral fibroblasts from HSF12 and HSF13 were measured following treatment with a range of DA receptor antagonists and agonists, administered 1 hour prior to the addition of DA. One experiment was conducted with three replicate wells for each compound tested, using two biological samples (HSF12 and HSF13; total n = 6). Results from the two cell lines were averaged and presented as mean ± SEM. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001 (two-way ANOVA).

    Article Snippet: The antibodies used were as follows: Dopamine Receptor D1 Rabbit mAb (381747; Zen-Bioscience), DRD2 polyclonal antibody (55084-1-AP; Proteintech, Rosemont, IL, USA), Dopamine Receptor D3 Rabbit mAb (382983; Zen-Bioscience), DRD4 Rabbit polyclonal antibody (28094-1-AP; Proteintech), Dopamine Receptor D5 Rabbit pAb (820522; Zen-Bioscience), GAPDH (7E4) Mouse mAb (200306-7E4; Zen-Bioscience), Beta Tubulin Polyclonal antibody (10094-1-AP; Proteintech), Goat anti-Rabbit IgG(H&L) (HRP conjugate) (511203; Zen-Bioscience), and Goat anti-Mouse IgG (H&L) (HRP conjugate) (511103; Zen-Bioscience).

    Techniques: Activity Assay

    Deregulated hippocampal GHSR and synaptic function in 24-month-old hAβ KI mice. A, B) Hippocampal GHSR level in (A) 14- and (B) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 3 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 200 μm (inset scale = 30 μm). C, D) Hippocampal GHSR/β-arrestin 2 complex level in (C) 14- and (D) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old nonTg n = 3 males, 2 females, hAβ KI n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). E, F) Hippocampal GHSR/DRD1 complex level in (E) 14- and (F) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). G, H) Hippocampal CamKII activation in (G) 14- and (H) 24-month-old hAβ KI mice and the nonTg controls represented by CamKII Thr286 phosphorylation. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females; 24-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females. Bottom panels are the representative images, scale bar = 30 μm. I, J) Hippocampal synaptic density in (I) 14- and (J) 24-month-old hAβ KI mice and the nonTg controls represented by the overlap of presynapse marker vGlut1 and postsynapse marker PSD95. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 2 males, 2 females; 24-month-old nonTg n = 2 males, 2 females; hAβ KI n = 2 males, 1 female. Bottom panels are the representative images, scale bar = 100 μm (inset scale = 10 μm). NS = not significant, *p < 0.05. Females: filled circles, males: open circles.

    Journal: Journal of Alzheimer's disease : JAD

    Article Title: Elevated Ghrelin Promotes Hippocampal Ghrelin Receptor Defects in Humanized Amyloid-β Knockin Mice During Aging

    doi: 10.3233/JAD-231002

    Figure Lengend Snippet: Deregulated hippocampal GHSR and synaptic function in 24-month-old hAβ KI mice. A, B) Hippocampal GHSR level in (A) 14- and (B) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 3 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 200 μm (inset scale = 30 μm). C, D) Hippocampal GHSR/β-arrestin 2 complex level in (C) 14- and (D) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old nonTg n = 3 males, 2 females, hAβ KI n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). E, F) Hippocampal GHSR/DRD1 complex level in (E) 14- and (F) 24-month-old hAβ KI mice and the nonTg controls. Unpaired two-way Student’s t test. 14-month-old n = 2 males, 2 females; 24-month-old n = 2 males, 2 females. Bottom panels are the representative images, scale bar = 250 μm (inset scale = 50 μm). G, H) Hippocampal CamKII activation in (G) 14- and (H) 24-month-old hAβ KI mice and the nonTg controls represented by CamKII Thr286 phosphorylation. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females; 24-month-old nonTg n = 2 males, 2 females, hAβ KI n = 3 males, 2 females. Bottom panels are the representative images, scale bar = 30 μm. I, J) Hippocampal synaptic density in (I) 14- and (J) 24-month-old hAβ KI mice and the nonTg controls represented by the overlap of presynapse marker vGlut1 and postsynapse marker PSD95. Unpaired two-way Student’s t test. 14-month-old nonTg n = 2 males, 2 females, hAβ KI n = 2 males, 2 females; 24-month-old nonTg n = 2 males, 2 females; hAβ KI n = 2 males, 1 female. Bottom panels are the representative images, scale bar = 100 μm (inset scale = 10 μm). NS = not significant, *p < 0.05. Females: filled circles, males: open circles.

    Article Snippet: The following primary antibodies were used in proper combinations: goat-anti-GHSR (Santa Cruz Biotechnology, #sc-10359, 1 : 100), rabbit-anti-DRD1 (Abcam, #ab81296, 1 : 200), mouse-anti -arrestin 2 (Santa Cruz, #sc-13140).

    Techniques: Activation Assay, Marker

    Western blots. A A typical Western blot for the D 1 receptor in hearts from WT, D 1 -TG, and D 1 -KO after incubation with the D 1 -dopamine receptor antibody is seen. The corresponding band for the D 1 receptor (DRD1) is labelled with an arrow. As loading control, the Ponceau S-stained membrane is shown below. B Typical Western blots for regulatory proteins in hearts from WT and D 1 -TG after incubation with the D 1 -dopamine receptor agonist SKF 38393 are seen. Western blots depict the phosphorylation state of inhibitory subunit of troponin (P-TnI) with arrows. As a loading control, we assessed the protein expression of cardiac calsequestrin (CSQ) by cutting horizontally the lanes of the blot and incubating the lower and upper halves with different primary antibodies. M rainbow marker, LA left atrium, RA right atrium, VT ventricle

    Journal: Naunyn-Schmiedeberg's Archives of Pharmacology

    Article Title: Initial characterization of a transgenic mouse with overexpression of the human D 1 -dopamine receptor in the heart

    doi: 10.1007/s00210-023-02901-y

    Figure Lengend Snippet: Western blots. A A typical Western blot for the D 1 receptor in hearts from WT, D 1 -TG, and D 1 -KO after incubation with the D 1 -dopamine receptor antibody is seen. The corresponding band for the D 1 receptor (DRD1) is labelled with an arrow. As loading control, the Ponceau S-stained membrane is shown below. B Typical Western blots for regulatory proteins in hearts from WT and D 1 -TG after incubation with the D 1 -dopamine receptor agonist SKF 38393 are seen. Western blots depict the phosphorylation state of inhibitory subunit of troponin (P-TnI) with arrows. As a loading control, we assessed the protein expression of cardiac calsequestrin (CSQ) by cutting horizontally the lanes of the blot and incubating the lower and upper halves with different primary antibodies. M rainbow marker, LA left atrium, RA right atrium, VT ventricle

    Article Snippet: First antibodies were rabbit polyclonal anti-calsequestrin (CSQ) antibody, #ab3516, Abcam, Cambridge, UK (diluted 1:20000), rabbit polyclonal anti-DRD1, #bs-1007R, Bioss, Woburn, MA, USA (dilution 1:500), and rabbit polyclonal anti-phospho-troponin I (P-TnI) antibody, #4004, Cell Signaling Technology Europe, Leiden, The Netherlands (diluted 1:5000).

    Techniques: Western Blot, Incubation, Control, Staining, Membrane, Expressing, Marker

    A Autoradiography. Representative images of autoradiography of D 1 -TG and WT mouse heart sections labeled with 5 nM [ 3 H]SCH23390 (total binding, TB) or 5 nM [ 3 H]SCH23390 + 10 M butaclamol (unspecific binding, UB). B In situ hybridization. Expression of D 1 -dopamine receptor mRNA detected by DIG-labelled human D 1 -dopamine receptor antisense probes (A-X) and DIG-labelled mouse D 1 -dopamine receptor antisense probes (a-l). DIG-labeled sense probes were used as controls. (A-H): Low magnification microscopic images, scale bar = 500 µm. mRNA expression of D 1 -dopamine receptor was not detected in WT mouse atria (A) and ventricles (C); whereas expression of human D 1 -dopamine receptor mRNA was detected in D 1 -Tg mouse atria (E) and ventricles including interventricular septum (G). (B, D, F, H) are corresponding control sections hybridized with DIG-labeled sense probes. (I-X): High magnification microscopic images, scale bar = 50 µm. No or very scarce and weak D 1 -dopamine mRNA expression was detected in WT mouse atria (I) and interventricular septum (K), while abundant human D 1 -dopamine mRNA expression was detected in atriums (M), interventricular septum (O), and ventricle walls (Q, S). (J, L, N, P, R, T) are corresponding control sections hybridized with DIG-labeled sense probes. D 1 -dopamine mRNA expression was also detected in human cardiomyocytes (U, W); while no signal was seen in corresponding control sections hybridized with DIG-labeled sense probes (V, X). (a-d): Low magnification microscopic images, scale bar = 500 µm. (e-h): High magnification microscopic images, scale bar = 50 µm. Expression of mouse D 1 -dopamine receptor mRNA was not detected in WT mouse atria (a, e) and ventricles (c, g); (b, d, f, h) are corresponding control sections hybridized with DIG-labeled sense probes. Low magnification images (i and j, scale bar = 500 µm) and high magnification images (k and l, scale bar = 50 µm) showed that the mouse antisense probe also detected human D 1 -dopamine mRNA expression in D 1 -TG mouse interventricular septum (i, k), while the mouse sense probe (control) did not detect any specific signal (j, l). C : Histology. Histological staining of myocardial sections with hematoxylin-eosin (HE) or Masson-Goldner trichome (MG) staining revealed no apparent abnormalities or signs of fibrosis, neither in WT nor in D 1 -TG. Scale bar = 100 µm. D : PCR. Scatter plots with means for the expression of exogenous transgenic D 1 -dopamine receptors (human-DRD1, left hand side) or endogenous mouse D 1 -dopamine receptors. Ordinates indicate the amount of the mRNA as inferred from the amplification cycles (Cq). *indicates significant differences between the mRNA from the whole heart of D 1 -TG versus WT

    Journal: Naunyn-Schmiedeberg's Archives of Pharmacology

    Article Title: Initial characterization of a transgenic mouse with overexpression of the human D 1 -dopamine receptor in the heart

    doi: 10.1007/s00210-023-02901-y

    Figure Lengend Snippet: A Autoradiography. Representative images of autoradiography of D 1 -TG and WT mouse heart sections labeled with 5 nM [ 3 H]SCH23390 (total binding, TB) or 5 nM [ 3 H]SCH23390 + 10 M butaclamol (unspecific binding, UB). B In situ hybridization. Expression of D 1 -dopamine receptor mRNA detected by DIG-labelled human D 1 -dopamine receptor antisense probes (A-X) and DIG-labelled mouse D 1 -dopamine receptor antisense probes (a-l). DIG-labeled sense probes were used as controls. (A-H): Low magnification microscopic images, scale bar = 500 µm. mRNA expression of D 1 -dopamine receptor was not detected in WT mouse atria (A) and ventricles (C); whereas expression of human D 1 -dopamine receptor mRNA was detected in D 1 -Tg mouse atria (E) and ventricles including interventricular septum (G). (B, D, F, H) are corresponding control sections hybridized with DIG-labeled sense probes. (I-X): High magnification microscopic images, scale bar = 50 µm. No or very scarce and weak D 1 -dopamine mRNA expression was detected in WT mouse atria (I) and interventricular septum (K), while abundant human D 1 -dopamine mRNA expression was detected in atriums (M), interventricular septum (O), and ventricle walls (Q, S). (J, L, N, P, R, T) are corresponding control sections hybridized with DIG-labeled sense probes. D 1 -dopamine mRNA expression was also detected in human cardiomyocytes (U, W); while no signal was seen in corresponding control sections hybridized with DIG-labeled sense probes (V, X). (a-d): Low magnification microscopic images, scale bar = 500 µm. (e-h): High magnification microscopic images, scale bar = 50 µm. Expression of mouse D 1 -dopamine receptor mRNA was not detected in WT mouse atria (a, e) and ventricles (c, g); (b, d, f, h) are corresponding control sections hybridized with DIG-labeled sense probes. Low magnification images (i and j, scale bar = 500 µm) and high magnification images (k and l, scale bar = 50 µm) showed that the mouse antisense probe also detected human D 1 -dopamine mRNA expression in D 1 -TG mouse interventricular septum (i, k), while the mouse sense probe (control) did not detect any specific signal (j, l). C : Histology. Histological staining of myocardial sections with hematoxylin-eosin (HE) or Masson-Goldner trichome (MG) staining revealed no apparent abnormalities or signs of fibrosis, neither in WT nor in D 1 -TG. Scale bar = 100 µm. D : PCR. Scatter plots with means for the expression of exogenous transgenic D 1 -dopamine receptors (human-DRD1, left hand side) or endogenous mouse D 1 -dopamine receptors. Ordinates indicate the amount of the mRNA as inferred from the amplification cycles (Cq). *indicates significant differences between the mRNA from the whole heart of D 1 -TG versus WT

    Article Snippet: First antibodies were rabbit polyclonal anti-calsequestrin (CSQ) antibody, #ab3516, Abcam, Cambridge, UK (diluted 1:20000), rabbit polyclonal anti-DRD1, #bs-1007R, Bioss, Woburn, MA, USA (dilution 1:500), and rabbit polyclonal anti-phospho-troponin I (P-TnI) antibody, #4004, Cell Signaling Technology Europe, Leiden, The Netherlands (diluted 1:5000).

    Techniques: Autoradiography, Labeling, Binding Assay, In Situ Hybridization, Expressing, Control, Staining, Transgenic Assay, Amplification

    Journal: Nature Communications

    Article Title: Non-canonical interplay between glutamatergic NMDA and dopamine receptors shapes synaptogenesis

    doi: 10.1038/s41467-023-44301-z

    Figure Lengend Snippet:

    Article Snippet: rabbit anti-D1R , 17934-1-AP , Proteintech , 2 μg.

    Techniques:

    HF, Hizikia fusiformis extract treatment; VEH, vehicle treatment (control); DRD1-5, dopamine D1–5 receptors; DAT, dopamine transporter; DAPI, 4′,6-diamidino-2-phenylindole; NF-L, neurofilament light chain; SERT, serotonin transporter; TH, tyrosine hydroxylase; TPH, tryptophan hydroxylase; SYP, synaptophysin; 5HT1A and 1B, serotonin 1A and 1B receptors; MAP2, microtubule-associated protein 2.

    Journal: Nutrition Research and Practice

    Article Title: Dopamine and serotonin alterations by Hizikia fusiformis extracts under in vitro cortical primary neuronal cell cultures

    doi: 10.4162/nrp.2023.17.3.408

    Figure Lengend Snippet: HF, Hizikia fusiformis extract treatment; VEH, vehicle treatment (control); DRD1-5, dopamine D1–5 receptors; DAT, dopamine transporter; DAPI, 4′,6-diamidino-2-phenylindole; NF-L, neurofilament light chain; SERT, serotonin transporter; TH, tyrosine hydroxylase; TPH, tryptophan hydroxylase; SYP, synaptophysin; 5HT1A and 1B, serotonin 1A and 1B receptors; MAP2, microtubule-associated protein 2.

    Article Snippet: In this study, we used primary antibodies for DA transmission: mouse monoclonal anti-tyrosine hydroxylase (TH; Abcam; catalog #ab129991), rabbit polyclonal anti-DAT (Santa Cruz; catalog #sc-14002), rabbit polyclonal anti-dopamine receptor D1 (DRD1; Santa Cruz; catalog #sc-14001), mouse monoclonal anti-DRD2 (Santa Cruz; catalog #sc-5303), mouse monoclonal anti-DRD3 (Santa Cruz; catalog #sc-136170), rabbit polyclonal anti-DRD4 (Elabscience; catalog #E-AB-31153), and rabbit polyclonal anti-DRD5 (Mybiosource; catalog #MBS2516950) antibodies; those for 5-HT transmission: rabbit polyclonal anti-5HT1A (Elabscience; catalog #E-AB-32950), rabbit polyclonal anti-5HT1B (Abcam; catalog #ab13896), anti-tryptophan hydroxylase (TPH; catalog #E-AB-16937), and mouse monoclonal anti-SERT (Santa Cruz; catalog #sc-33724) antibodies; and those for neuronal structures: mouse monoclonal anti-synaptophysin (SYP; Sigma-Aldrich; catalog #S5768), mouse monoclonal anti-microtubule-associated protein 2 (MAP2; Santa Cruz; catalog #sc-32791), and mouse monoclonal neurofilament-light chain (NF-L; Santa Cruz; catalog #sc-20012) antibodies.

    Techniques:

    DRD1–5, dopamine D1–5 receptors; HF, Hizikia fusiformis extract treatment; VEH, vehicle treatment (control); DAT, dopamine transporter; TH, tyrosine hydroxylase.

    Journal: Nutrition Research and Practice

    Article Title: Dopamine and serotonin alterations by Hizikia fusiformis extracts under in vitro cortical primary neuronal cell cultures

    doi: 10.4162/nrp.2023.17.3.408

    Figure Lengend Snippet: DRD1–5, dopamine D1–5 receptors; HF, Hizikia fusiformis extract treatment; VEH, vehicle treatment (control); DAT, dopamine transporter; TH, tyrosine hydroxylase.

    Article Snippet: In this study, we used primary antibodies for DA transmission: mouse monoclonal anti-tyrosine hydroxylase (TH; Abcam; catalog #ab129991), rabbit polyclonal anti-DAT (Santa Cruz; catalog #sc-14002), rabbit polyclonal anti-dopamine receptor D1 (DRD1; Santa Cruz; catalog #sc-14001), mouse monoclonal anti-DRD2 (Santa Cruz; catalog #sc-5303), mouse monoclonal anti-DRD3 (Santa Cruz; catalog #sc-136170), rabbit polyclonal anti-DRD4 (Elabscience; catalog #E-AB-31153), and rabbit polyclonal anti-DRD5 (Mybiosource; catalog #MBS2516950) antibodies; those for 5-HT transmission: rabbit polyclonal anti-5HT1A (Elabscience; catalog #E-AB-32950), rabbit polyclonal anti-5HT1B (Abcam; catalog #ab13896), anti-tryptophan hydroxylase (TPH; catalog #E-AB-16937), and mouse monoclonal anti-SERT (Santa Cruz; catalog #sc-33724) antibodies; and those for neuronal structures: mouse monoclonal anti-synaptophysin (SYP; Sigma-Aldrich; catalog #S5768), mouse monoclonal anti-microtubule-associated protein 2 (MAP2; Santa Cruz; catalog #sc-32791), and mouse monoclonal neurofilament-light chain (NF-L; Santa Cruz; catalog #sc-20012) antibodies.

    Techniques:

    A summary of BF 10 with post-hoc pair wise comparisons

    Journal: Nutrition Research and Practice

    Article Title: Dopamine and serotonin alterations by Hizikia fusiformis extracts under in vitro cortical primary neuronal cell cultures

    doi: 10.4162/nrp.2023.17.3.408

    Figure Lengend Snippet: A summary of BF 10 with post-hoc pair wise comparisons

    Article Snippet: In this study, we used primary antibodies for DA transmission: mouse monoclonal anti-tyrosine hydroxylase (TH; Abcam; catalog #ab129991), rabbit polyclonal anti-DAT (Santa Cruz; catalog #sc-14002), rabbit polyclonal anti-dopamine receptor D1 (DRD1; Santa Cruz; catalog #sc-14001), mouse monoclonal anti-DRD2 (Santa Cruz; catalog #sc-5303), mouse monoclonal anti-DRD3 (Santa Cruz; catalog #sc-136170), rabbit polyclonal anti-DRD4 (Elabscience; catalog #E-AB-31153), and rabbit polyclonal anti-DRD5 (Mybiosource; catalog #MBS2516950) antibodies; those for 5-HT transmission: rabbit polyclonal anti-5HT1A (Elabscience; catalog #E-AB-32950), rabbit polyclonal anti-5HT1B (Abcam; catalog #ab13896), anti-tryptophan hydroxylase (TPH; catalog #E-AB-16937), and mouse monoclonal anti-SERT (Santa Cruz; catalog #sc-33724) antibodies; and those for neuronal structures: mouse monoclonal anti-synaptophysin (SYP; Sigma-Aldrich; catalog #S5768), mouse monoclonal anti-microtubule-associated protein 2 (MAP2; Santa Cruz; catalog #sc-32791), and mouse monoclonal neurofilament-light chain (NF-L; Santa Cruz; catalog #sc-20012) antibodies.

    Techniques: