Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue

The sigma 1 receptor (S1R) is widely expressed in the CNS and is mainly located on the endoplasmic reticulum. The S1R is involved in the regulation of many neurotransmission systems and, indirectly, in neurodegenerative diseases. The S1R may therefore represent an interesting neuronal biomarker in n...

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Autores principales: Lepelletier, François-Xavier, Vandesquille, Matthias, Asselin, Marie-Claude, Prenant, Christian, Robinson, Andrew C, Mann, David M A, Green, Michael, Barnett, Elizabeth, Banister, Samuel D, Mottinelli, Marco, Mesangeau, Christophe, McCurdy, Christopher R, Fricke, Inga B, Jacobs, Andreas H., Kassiou, Michael, Boutin, Hervé
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Ivyspring International Publisher 2020
Materias:
Research Paper
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7381740/
https://www.ncbi.nlm.nih.gov/pubmed/32724451
http://dx.doi.org/10.7150/thno.47585
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author Lepelletier, François-Xavier
Vandesquille, Matthias
Asselin, Marie-Claude
Prenant, Christian
Robinson, Andrew C
Mann, David M A
Green, Michael
Barnett, Elizabeth
Banister, Samuel D
Mottinelli, Marco
Mesangeau, Christophe
McCurdy, Christopher R
Fricke, Inga B
Jacobs, Andreas H.
Kassiou, Michael
Boutin, Hervé
author_facet Lepelletier, François-Xavier
Vandesquille, Matthias
Asselin, Marie-Claude
Prenant, Christian
Robinson, Andrew C
Mann, David M A
Green, Michael
Barnett, Elizabeth
Banister, Samuel D
Mottinelli, Marco
Mesangeau, Christophe
McCurdy, Christopher R
Fricke, Inga B
Jacobs, Andreas H.
Kassiou, Michael
Boutin, Hervé
author_sort Lepelletier, François-Xavier
collection PubMed
description The sigma 1 receptor (S1R) is widely expressed in the CNS and is mainly located on the endoplasmic reticulum. The S1R is involved in the regulation of many neurotransmission systems and, indirectly, in neurodegenerative diseases. The S1R may therefore represent an interesting neuronal biomarker in neurodegenerative diseases such as Parkinson's (PD) or Alzheimer's diseases (AD). Here we present the characterisation of the S1R-specific (18)F-labelled tracer (18)F-IAM6067 in two animal models and in human brain tissue. Methods: Wistar rats were used for PET-CT imaging (60 min dynamic acquisition) and metabolite analysis (1, 2, 5, 10, 20, 60 min post-injection). To verify in vivo selectivity, haloperidol, BD1047 (S1R ligand), CM398 (S2R ligand) and SB206553 (5HT(2B/C) antagonist) were administrated for pre-saturation studies. Excitotoxic lesions induced by intra-striatal injection of AMPA were also imaged by (18)F-IAM6067 PET-CT to test the sensitivity of the methods in a well-established model of neuronal loss. Tracer brain uptake was also verified by autoradiography in rats and in a mouse model of PD (intrastriatal 6-hydroxydopamine (6-OHDA) unilateral lesion). Finally, human cortical binding was investigated by autoradiography in three groups of subjects (control subjects with Braak ≤2, and AD patients, Braak >2 & ≤4 and Braak >4 stages). Results: We demonstrate that despite rapid peripheral metabolism of (18)F-IAM6067, radiolabelled metabolites were hardly detected in brain samples. Brain uptake of (18)F-IAM6067 showed differences in S1R anatomical distribution, namely from high to low uptake: pons-raphe, thalamus medio-dorsal, substantia nigra, hypothalamus, cerebellum, cortical areas and striatum. Pre-saturation studies showed 79-90% blockade of the binding in all areas of the brain indicated above except with the 5HT(2B/C) antagonist SB206553 and S2R ligand CM398 which induced no significant blockade, indicating good specificity of (18)F-IAM6067 for S1Rs. No difference between ipsi- and contralateral sides of the brain in the mouse model of PD was detected. AMPA lesion induced a significant 69% decrease in (18)F-IAM6067 uptake in the globus pallidus matching the neuronal loss as measured by NeuN, but only a trend to decrease (-16%) in the caudate putamen despite a significant 91% decrease in neuronal count. Moreover, no difference in the human cortical binding was shown between AD groups and controls. Conclusion: This work shows that (18)F-IAM6067 is a specific and selective S1R radiotracer. The absence or small changes in S1R detected here in animal models and human tissue warrants further investigations and suggests that S1R might not be the anticipated ideal biomarker for neuronal loss in neurodegenerative diseases such as AD and PD.
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spelling pubmed-73817402020-07-27 Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue Lepelletier, François-Xavier Vandesquille, Matthias Asselin, Marie-Claude Prenant, Christian Robinson, Andrew C Mann, David M A Green, Michael Barnett, Elizabeth Banister, Samuel D Mottinelli, Marco Mesangeau, Christophe McCurdy, Christopher R Fricke, Inga B Jacobs, Andreas H. Kassiou, Michael Boutin, Hervé Theranostics Research Paper The sigma 1 receptor (S1R) is widely expressed in the CNS and is mainly located on the endoplasmic reticulum. The S1R is involved in the regulation of many neurotransmission systems and, indirectly, in neurodegenerative diseases. The S1R may therefore represent an interesting neuronal biomarker in neurodegenerative diseases such as Parkinson's (PD) or Alzheimer's diseases (AD). Here we present the characterisation of the S1R-specific (18)F-labelled tracer (18)F-IAM6067 in two animal models and in human brain tissue. Methods: Wistar rats were used for PET-CT imaging (60 min dynamic acquisition) and metabolite analysis (1, 2, 5, 10, 20, 60 min post-injection). To verify in vivo selectivity, haloperidol, BD1047 (S1R ligand), CM398 (S2R ligand) and SB206553 (5HT(2B/C) antagonist) were administrated for pre-saturation studies. Excitotoxic lesions induced by intra-striatal injection of AMPA were also imaged by (18)F-IAM6067 PET-CT to test the sensitivity of the methods in a well-established model of neuronal loss. Tracer brain uptake was also verified by autoradiography in rats and in a mouse model of PD (intrastriatal 6-hydroxydopamine (6-OHDA) unilateral lesion). Finally, human cortical binding was investigated by autoradiography in three groups of subjects (control subjects with Braak ≤2, and AD patients, Braak >2 & ≤4 and Braak >4 stages). Results: We demonstrate that despite rapid peripheral metabolism of (18)F-IAM6067, radiolabelled metabolites were hardly detected in brain samples. Brain uptake of (18)F-IAM6067 showed differences in S1R anatomical distribution, namely from high to low uptake: pons-raphe, thalamus medio-dorsal, substantia nigra, hypothalamus, cerebellum, cortical areas and striatum. Pre-saturation studies showed 79-90% blockade of the binding in all areas of the brain indicated above except with the 5HT(2B/C) antagonist SB206553 and S2R ligand CM398 which induced no significant blockade, indicating good specificity of (18)F-IAM6067 for S1Rs. No difference between ipsi- and contralateral sides of the brain in the mouse model of PD was detected. AMPA lesion induced a significant 69% decrease in (18)F-IAM6067 uptake in the globus pallidus matching the neuronal loss as measured by NeuN, but only a trend to decrease (-16%) in the caudate putamen despite a significant 91% decrease in neuronal count. Moreover, no difference in the human cortical binding was shown between AD groups and controls. Conclusion: This work shows that (18)F-IAM6067 is a specific and selective S1R radiotracer. The absence or small changes in S1R detected here in animal models and human tissue warrants further investigations and suggests that S1R might not be the anticipated ideal biomarker for neuronal loss in neurodegenerative diseases such as AD and PD. Ivyspring International Publisher 2020-06-29 /pmc/articles/PMC7381740/ /pubmed/32724451 http://dx.doi.org/10.7150/thno.47585 Text en © The author(s) This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/). See http://ivyspring.com/terms for full terms and conditions.
spellingShingle Research Paper
Lepelletier, François-Xavier
Vandesquille, Matthias
Asselin, Marie-Claude
Prenant, Christian
Robinson, Andrew C
Mann, David M A
Green, Michael
Barnett, Elizabeth
Banister, Samuel D
Mottinelli, Marco
Mesangeau, Christophe
McCurdy, Christopher R
Fricke, Inga B
Jacobs, Andreas H.
Kassiou, Michael
Boutin, Hervé
Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title_full Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title_fullStr Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title_full_unstemmed Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title_short Evaluation of (18)F-IAM6067 as a sigma-1 receptor PET tracer for neurodegeneration in vivo in rodents and in human tissue
title_sort evaluation of (18)f-iam6067 as a sigma-1 receptor pet tracer for neurodegeneration in vivo in rodents and in human tissue
topic Research Paper
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC7381740/
https://www.ncbi.nlm.nih.gov/pubmed/32724451
http://dx.doi.org/10.7150/thno.47585
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