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GenScript corporation mouse 5-ht 3a r gene
Mouse 5 Ht 3a R Gene, supplied by GenScript corporation, 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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mouse 5-ht 3a r gene - by Bioz Stars, 2026-03

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Cryogenic electron microscopy (cryo-EM) structure of granisetron-bound full-length serotonin 3A receptor (5-HT 3A R). a A schematic showing three fundamental conformations that constitute the gating cycle in pentameric ligand-gated ion channel (pLGIC) function: a resting state, a transient open state, and a desensitized state. Agonist-binding shifts the equilibrium towards the open state and then to the high-agonist affinity, desensitized state. Orthosteric (competitive) antagonists exert their effect by shifting the equilibrium towards the resting (or inhibited) state. b Trace showing a continuous recording of 5-HT <t>3A</t> <t>R</t> currents (−60 mV) in oocytes measured by two-electrode voltage clamp (TEVC) in the presence of serotonin (marked by red line) and pre-applied granisetron (marked by orange line). The effect of granisetron inhibition was fully reversible as seen in the third pulse. c Map of full-length 5-HT 3A R-granisetron reconstructed from 46,757 particles at 2.92 Å resolution. Side-view parallel to the membrane and extracellular view are shown in left and right panels, respectively. Each monomer is shown in a different color for clarity. Density corresponding to granisetron (left panel, circle) and glycans (right panel, arrow) are indicated. d Three-dimensional cartoon model of 5-HT 3A R-granisetron structure generated from EM reconstruction (side view). For each subunit, three sets of glycans are shown as stick representation. e Top-view of 5-HT 3A R-granisetron map sliced at the binding site to show all five granisetron molecules, each bound at the interface of two subunits (indicated by arrows)

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Sequence of mouse 5-HT <t> 3A R </t> used in the cryo-EM study and the data on cryo-EM and refinement. a, Full length mouse 5-HT <t> 3A R </t> sequence used in the cryo-EM study. Regions in the sequence highlighted in green, blue, gray, and yellow represent strep-tag, linker, TEV cleavage site, and 1D4-tag, respectively. Secondary structural elements as seen in State 1 are plotted above the sequence. Loops in gray color are not seen in the final refined structure. All the important loops, sheets, and helices are labeled. Glycosylation sites are marked as blue arrows. Key residues within the serotonin-binding sites are highlighted in brown color. Cysteines present in the cys-loop are shown as cyan color. Pore-facing residues in M2 are shown in green color. Arg416 in the ICD is shown in red. b, Cryo-EM data collection, refinement and validation statistics.

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Image Search Results

Journal: Nature Communications

Article Title: Molecular mechanism of setron-mediated inhibition of full-length 5-HT 3A receptor

doi: 10.1038/s41467-019-11142-8

Figure Lengend Snippet: Cryogenic electron microscopy (cryo-EM) structure of granisetron-bound full-length serotonin 3A receptor (5-HT 3A R). a A schematic showing three fundamental conformations that constitute the gating cycle in pentameric ligand-gated ion channel (pLGIC) function: a resting state, a transient open state, and a desensitized state. Agonist-binding shifts the equilibrium towards the open state and then to the high-agonist affinity, desensitized state. Orthosteric (competitive) antagonists exert their effect by shifting the equilibrium towards the resting (or inhibited) state. b Trace showing a continuous recording of 5-HT 3A R currents (−60 mV) in oocytes measured by two-electrode voltage clamp (TEVC) in the presence of serotonin (marked by red line) and pre-applied granisetron (marked by orange line). The effect of granisetron inhibition was fully reversible as seen in the third pulse. c Map of full-length 5-HT 3A R-granisetron reconstructed from 46,757 particles at 2.92 Å resolution. Side-view parallel to the membrane and extracellular view are shown in left and right panels, respectively. Each monomer is shown in a different color for clarity. Density corresponding to granisetron (left panel, circle) and glycans (right panel, arrow) are indicated. d Three-dimensional cartoon model of 5-HT 3A R-granisetron structure generated from EM reconstruction (side view). For each subunit, three sets of glycans are shown as stick representation. e Top-view of 5-HT 3A R-granisetron map sliced at the binding site to show all five granisetron molecules, each bound at the interface of two subunits (indicated by arrows)

Article Snippet: Codon-optimized mouse 5-HT 3A R (NCBI Reference Sequence: NM_001099644.1) was purchased from GenScript (Supplementary Table ) and inserted into pFastBac1 vector consisting of four strep-tags (WSHPQFEK) at the N terminus, followed by a linker sequence (GGGSGGGSGGGS) and a TEV-cleavage sequence (ENLYFQG) and a C-terminal 1D4-tag .

Techniques: Electron Microscopy, Cryo-EM Sample Prep, Binding Assay, Inhibition, Generated

The granisetron binding site. a The density map of granisetron contoured at 9 σ (left) and map around the residues at the binding site located at the intersubunit interface (right). The residue labels on the principal subunit are marked in black and those on the complementary subunit are marked in brown. b A comparison of the serotonin 3A receptor-apo (5-HT 3A R-apo), 5-HT 3A R-granisetron, and 5-HT 3A R-serotonin structures shows that residues involved in ligand-binding undergo rotameric reorientation. c Alignment of the three structures reveals an inward motion of loop C in 5-HT 3A R-granisetron relative to 5-HT 3A R-apo, which is in the direction toward activation as seen in the 5-HT 3A R-serotonin structure

Journal: Nature Communications

Article Title: Molecular mechanism of setron-mediated inhibition of full-length 5-HT 3A receptor

doi: 10.1038/s41467-019-11142-8

Figure Lengend Snippet: The granisetron binding site. a The density map of granisetron contoured at 9 σ (left) and map around the residues at the binding site located at the intersubunit interface (right). The residue labels on the principal subunit are marked in black and those on the complementary subunit are marked in brown. b A comparison of the serotonin 3A receptor-apo (5-HT 3A R-apo), 5-HT 3A R-granisetron, and 5-HT 3A R-serotonin structures shows that residues involved in ligand-binding undergo rotameric reorientation. c Alignment of the three structures reveals an inward motion of loop C in 5-HT 3A R-granisetron relative to 5-HT 3A R-apo, which is in the direction toward activation as seen in the 5-HT 3A R-serotonin structure

Techniques: Binding Assay, Ligand Binding Assay, Activation Assay

Conformational differences between the apo and ligand-bound states. a An extracellular view of the extracellular domain (ECD) upon global alignment of serotonin 3A receptor-apo (5-HT 3A R-apo) structure with 5-HT 3A R-granisetron (left) and 5-HT 3A R-serotonin (right). Only ECDs from two non-adjacent subunits is shown for clarity. A counter-clockwise motion of the ECD is observed as indicated by the arrows. The serotonin-induced motion is of larger magnitude compared to that of granisetron, highlighted by the solid and dotted arrows, respectively. b A comparison of the transmembrane domains (TMDs) (viewed from the extracellular side) in 5-HT 3A R-granisetron structure (left) and 5-HT 3A R-serotonin (right) when aligned with respect to 5-HT 3A R-apo. Only two non-adjacent TMD subunits are shown for clarity. In both panels, a clockwise rotation of the TMD is observed with 5-HT 3A R-serotonin revealing a larger change. c Pathway of ion permeation of 5-HT 3A R-apo and 5-HT 3A R-granisetron generated with HOLE . The cartoon representation of two subunits are shown for clarity. The locations of pore constrictions are shown as sticks. The pore radius is plotted as a function of distance along the pore axis. The dotted line indicates the approximate radius of a hydrated Na + ion, which is estimated at 2.76 Å (right)

Journal: Nature Communications

Article Title: Molecular mechanism of setron-mediated inhibition of full-length 5-HT 3A receptor

doi: 10.1038/s41467-019-11142-8

Figure Lengend Snippet: Conformational differences between the apo and ligand-bound states. a An extracellular view of the extracellular domain (ECD) upon global alignment of serotonin 3A receptor-apo (5-HT 3A R-apo) structure with 5-HT 3A R-granisetron (left) and 5-HT 3A R-serotonin (right). Only ECDs from two non-adjacent subunits is shown for clarity. A counter-clockwise motion of the ECD is observed as indicated by the arrows. The serotonin-induced motion is of larger magnitude compared to that of granisetron, highlighted by the solid and dotted arrows, respectively. b A comparison of the transmembrane domains (TMDs) (viewed from the extracellular side) in 5-HT 3A R-granisetron structure (left) and 5-HT 3A R-serotonin (right) when aligned with respect to 5-HT 3A R-apo. Only two non-adjacent TMD subunits are shown for clarity. In both panels, a clockwise rotation of the TMD is observed with 5-HT 3A R-serotonin revealing a larger change. c Pathway of ion permeation of 5-HT 3A R-apo and 5-HT 3A R-granisetron generated with HOLE . The cartoon representation of two subunits are shown for clarity. The locations of pore constrictions are shown as sticks. The pore radius is plotted as a function of distance along the pore axis. The dotted line indicates the approximate radius of a hydrated Na + ion, which is estimated at 2.76 Å (right)

Techniques: Generated

Assessment of the overall stability of the granisetron-serotonin 3A receptor (5-HT 3A R) structure. a Time evolution of the root mean squared deviations (RMSD) of Cα atoms of secondary structure elements of the extracellular domain (ECD) and all Cα atoms of the 5-HT 3A R pentamer (left panel). The RMSD of each of the granisetron molecules (labeled CWB) in each subunit A to E (right panel) calculated with respect to the cryo-EM-derived structure during 100 ns production simulations. b Two possible granisetron poses with the bicyclic ring in boat/chair or chair/chair conformation and the N -methyl group in axial or equatorial positions in the piperidine chair conformation. These two poses were used as input for metadynamics-based ranking. c Ranking of the two granisetron poses shown in b using metadynamics. Error bars represent the standard error of the mean of RMSD estimates from 10 metadynamics simulations. Source data are provided as a

Journal: Nature Communications

Article Title: Molecular mechanism of setron-mediated inhibition of full-length 5-HT 3A receptor

doi: 10.1038/s41467-019-11142-8

Figure Lengend Snippet: Assessment of the overall stability of the granisetron-serotonin 3A receptor (5-HT 3A R) structure. a Time evolution of the root mean squared deviations (RMSD) of Cα atoms of secondary structure elements of the extracellular domain (ECD) and all Cα atoms of the 5-HT 3A R pentamer (left panel). The RMSD of each of the granisetron molecules (labeled CWB) in each subunit A to E (right panel) calculated with respect to the cryo-EM-derived structure during 100 ns production simulations. b Two possible granisetron poses with the bicyclic ring in boat/chair or chair/chair conformation and the N -methyl group in axial or equatorial positions in the piperidine chair conformation. These two poses were used as input for metadynamics-based ranking. c Ranking of the two granisetron poses shown in b using metadynamics. Error bars represent the standard error of the mean of RMSD estimates from 10 metadynamics simulations. Source data are provided as a

Techniques: Labeling, Cryo-EM Sample Prep, Derivative Assay

Effects of mutations at the ligand-binding pocket on granisetron inhibition. a Granisetron interactions with Trp156 and Tyr207 from the principal subunit and Trp63, Arg65, Tyr126 from the complementary subunit are depicted as stick representation. b Serotonin dose response measured by two-electrode voltage clamp (TEVC) recordings (at −60 mV) for wild-type (WT) 5-HT 3A R, W63Y, R65A, Y126F, W156Y, and Y207F mutants, expressed in oocytes. The half-maximal effective concentration (EC 50 ), the Hill coefficient (nH), and the number of independent oocyte experiments for WT and mutants are: WT (EC 50 : 2.70 + 0.09 μM; nH: 2.3 + 0.17; n: 3), W63Y (EC 50 : 9.93 + 0.77 μM; nH: 3.1 + 0.72; n: 4), R65A (EC 50 : 13.79 + 0.50 μM; nH: 4.4 + 0.59; n: 4), Y126F (EC 50 : 42.8 + 4.4 μM; nH: 2.6 + 0.71; n: 4), W156Y (EC 50 : 306 + 44 μM; nH: 1.58 + 0.24; n: 4), and Y207F (EC 50 : 20.35 + 1.7 μM; nH: 1.9 + 0.27; n: 5). c Currents were elicited in response to serotonin (concentrations used near EC 50 values of WT and mutants). The following concentrations of serotonin were used: WT-1 μM, W63Y-10 μM, R65A-10 μM; Y126F-40 μM, W156Y-200 μM, and Y207F-20 μM. Currents were measured in response to serotonin (marked by red line) and pre-application of granisetron (marked by orange line). Dotted arrows show the extent of granisetron inhibition. d A plot of the ratio of peak current in the presence of granisetron to peak current in the absence of granisetron is shown for WT and mutants. Data are shown as mean ± s.d. (n is indicated within parentheses). Significance at p = 0.001 (***) and p = 0.05 (**) calculated by two-sample t test for WT and mutants. Source data are provided as a

Journal: Nature Communications

Article Title: Molecular mechanism of setron-mediated inhibition of full-length 5-HT 3A receptor

doi: 10.1038/s41467-019-11142-8

Figure Lengend Snippet: Effects of mutations at the ligand-binding pocket on granisetron inhibition. a Granisetron interactions with Trp156 and Tyr207 from the principal subunit and Trp63, Arg65, Tyr126 from the complementary subunit are depicted as stick representation. b Serotonin dose response measured by two-electrode voltage clamp (TEVC) recordings (at −60 mV) for wild-type (WT) 5-HT 3A R, W63Y, R65A, Y126F, W156Y, and Y207F mutants, expressed in oocytes. The half-maximal effective concentration (EC 50 ), the Hill coefficient (nH), and the number of independent oocyte experiments for WT and mutants are: WT (EC 50 : 2.70 + 0.09 μM; nH: 2.3 + 0.17; n: 3), W63Y (EC 50 : 9.93 + 0.77 μM; nH: 3.1 + 0.72; n: 4), R65A (EC 50 : 13.79 + 0.50 μM; nH: 4.4 + 0.59; n: 4), Y126F (EC 50 : 42.8 + 4.4 μM; nH: 2.6 + 0.71; n: 4), W156Y (EC 50 : 306 + 44 μM; nH: 1.58 + 0.24; n: 4), and Y207F (EC 50 : 20.35 + 1.7 μM; nH: 1.9 + 0.27; n: 5). c Currents were elicited in response to serotonin (concentrations used near EC 50 values of WT and mutants). The following concentrations of serotonin were used: WT-1 μM, W63Y-10 μM, R65A-10 μM; Y126F-40 μM, W156Y-200 μM, and Y207F-20 μM. Currents were measured in response to serotonin (marked by red line) and pre-application of granisetron (marked by orange line). Dotted arrows show the extent of granisetron inhibition. d A plot of the ratio of peak current in the presence of granisetron to peak current in the absence of granisetron is shown for WT and mutants. Data are shown as mean ± s.d. (n is indicated within parentheses). Significance at p = 0.001 (***) and p = 0.05 (**) calculated by two-sample t test for WT and mutants. Source data are provided as a

Techniques: Ligand Binding Assay, Inhibition, Concentration Assay

Sequence of mouse 5-HT 3A R used in the cryo-EM study and the data on cryo-EM and refinement. a, Full length mouse 5-HT 3A R sequence used in the cryo-EM study. Regions in the sequence highlighted in green, blue, gray, and yellow represent strep-tag, linker, TEV cleavage site, and 1D4-tag, respectively. Secondary structural elements as seen in State 1 are plotted above the sequence. Loops in gray color are not seen in the final refined structure. All the important loops, sheets, and helices are labeled. Glycosylation sites are marked as blue arrows. Key residues within the serotonin-binding sites are highlighted in brown color. Cysteines present in the cys-loop are shown as cyan color. Pore-facing residues in M2 are shown in green color. Arg416 in the ICD is shown in red. b, Cryo-EM data collection, refinement and validation statistics.

Journal: Nature

Article Title: Cryo-EM reveals two distinct serotonin-bound conformations of full-length 5-HT 3A receptor

doi: 10.1038/s41586-018-0660-7

Figure Lengend Snippet: Sequence of mouse 5-HT 3A R used in the cryo-EM study and the data on cryo-EM and refinement. a, Full length mouse 5-HT 3A R sequence used in the cryo-EM study. Regions in the sequence highlighted in green, blue, gray, and yellow represent strep-tag, linker, TEV cleavage site, and 1D4-tag, respectively. Secondary structural elements as seen in State 1 are plotted above the sequence. Loops in gray color are not seen in the final refined structure. All the important loops, sheets, and helices are labeled. Glycosylation sites are marked as blue arrows. Key residues within the serotonin-binding sites are highlighted in brown color. Cysteines present in the cys-loop are shown as cyan color. Pore-facing residues in M2 are shown in green color. Arg416 in the ICD is shown in red. b, Cryo-EM data collection, refinement and validation statistics.

Article Snippet: Codon optimized mouse 5-HT 3A R gene (NCBI Reference Sequence: NM_001099644.1 ) was purchased from GenScript USA Inc and subcloned into pFastBac1 vector.

Techniques: Sequencing, Strep-tag, Labeling, Glycoproteomics, Biomarker Discovery