| Literature DB >> 31079591 |
Danielly Chierrito1, Camila B Villas-Boas2, Fernanda S Tonin3, Fernando Fernandez-Llimos4, Andréia C C Sanches2, João C P de Mello1.
Abstract
BACKGROUND: Advances in basic and molecular biology have promoted the use of cell cultures in a wide range of areas, including the evaluation of drug efficacy, safety and toxicity.Entities:
Keywords: ADHD; ADHD treatment; Cell model; checklist; flowchart; methodological aspect; neuronal cell.
Mesh:
Substances:
Year: 2019 PMID: 31079591 PMCID: PMC7052832 DOI: 10.2174/1570159X17666190409143155
Source DB: PubMed Journal: Curr Neuropharmacol ISSN: 1570-159X Impact factor: 7.363
Main characteristics of all the studies included in the systematic review.
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| Schmidt | Germany | SH-SY5Y, | Amphetamine, Atomoxetine, | A, C |
| Schmidt | Germany | SH-SY5Y, | Amphetamine, Atomoxetine, | A, B |
| Schmidt | Germany | SH-SY5Y |
| A, B |
| Nam | Korea | SH-SY5Y | YY162* | A |
| Feio-Azevedo | Portugal | SH-SY5Y | Amphetamine e metabolites** | A, C |
| Bartl | Germany | PC12 | Methylphenidate | A, B, C |
| Bartl | Switzerland | PC12 | Polyunsaturated fatty acids | A, B |
| Craenenbroeck | Belgium | HEK293rtTA, L929sA, CHO | Pipamperone | A, C |
| Wakamatsu | Japan | HEK-293 | Methylphenidate | A |
| Ludolph | Germany | TsA201 | Atomoxetine | A |
| Knorle | Germany | JAR |
| A, B |
| Suter | Switzerland | Human lymphocytes | Methylphenidate | A |
| Schwarz | Germany | Lymphoblastoid cell lines | Methylphenidate | A, C |
| Kittel-Schneider | Germany | Peripheral blood mononuclear cells | Methylphenidate | A |
| Zhao | China | CHO |
| A |
| Salviano | Brazil | MDCK | Methylphenidate | A, B |
Abbreviations: SH-SY5Y: neuroblastoma SH-SY5Y; U-937: Human monocytic U-927; PC12: Rat pheochromocytoma; HEK293rtTA cells: Human embryonic kidney cells expressing the tetracycline transactivator; HEK-293: Human embryonic kidney 293; TsA201: Transformed human embryonic kidney; JAR: Human choriocarcinoma; L929sA: pMx5-HT2AR cells mouse fibrosarcoma; CHO: Chinese hamster ovary; MDCK: Madin-darby canine kidney; *YY162: Mixture of “terpenoid-strengthened Ginkgo biloba” and “ginsenoside Rg3”; **4-hydroxyamphetamine e 4-hydroxynorephedrine; A: culture conditions; B: cell viability; C: gene expression.
Main tests reported in the studies with non-neuronal cells cultures.
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| Craenenbroeck | HEK293rtTA | To evaluate the effect of pipamperone on D4 receptor expression | - | qPCR | Radioligant Western blot |
| Wakamatsu | HEK 293 | To evalute the effect of methylphenidate on the cardiovascular system | - | - | Electro-physiological |
| Ludolph | TsA201 | To evaluate the effect of atomoxetine on glutamate receptors | - | - | Electro-physiological |
| Knorle | JAR | To evaluate the effect of | LDH | - | Effect on transporters |
| Suter | Human | To evaluate the clastogenic effect of methylphenidate | - | - | Chromosome |
| Schwarz | Lymphoblastoid Cell Lines | To evaluate the effect of methylphenidate on gene expression regulation | - | qRT-PCR | - |
| Kittel-Schneider | Peripheral blood mononuclear cells | To evaluate the cytogenetic effects of long-term treatment with methylphenidate | - | - | Micronucleus |
| Craenenbroeck | L929sA | To evaluate the effect of pipamperone on D4 receptor expression | qPCR | Radioligant | |
| Craenenbroeck | CHO | To evaluate the effect of pipamperone on D4 receptor expression | - | qPCR | Radioligant |
| Zhao | CHO | To evaluate the effect of | - | - | Effect on transporters |
| Salviano | MDCK | Evaluate the effect of methylphenidate on the renal system | MTT | - | - |
Abbreviations: HEK293rtTA cells: Human embryonic kidney cells expressing the tetracycline transactivator HEK-293: Human Embryonic Kidney; TsA201: Transformed human embryonic kidney; JAR: Human choriocarcinoma; L929sA: Cells mouse fibrosarcoma; CHO: Chinese Hamster Ovary; MDCK: Madin-Darby Canine Kidney; Receptor D4: Receptor de dopamine 4; 6-OHDA: 6-hydroxydopamine; qRT-PCR: quantitative Real Time PCR; *Eicosapentaenoic acid e docosahexanoic acid e gamma-linolenic acid.
Checklist for conduct and reporting experimental in vitro studies.
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| Identification of culture type | |
| Identification of cell type | |
| Origin of cells (human, animal) | |
| In case of cells isolated from tissues, report isolation technique and variables involved | |
| Source of access of cells (collection of cell biology, donation by laboratories) | |
| In case of collection of cell biology, report the product/catalog number | |
| Growth medium used | |
| Growth medium supplementation components (serum, antibiotics, micronutrients, others). Report name, concentration, percentage used and brand | |
| Frequency of change of growth medium | |
| pH of the growth medium | |
| Confluence | |
| Use of trypsin or other substance to collect the cells. Report name, concentration, percentage | |
| Cellular density | |
| Number of passages | |
| Incubation temperature (exact 0.0 °C) | |
| Atmosphere conditions (exact 0.0% CO2) | |
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| Technique name | |
| Report whether the technique has been developed and validated or reproduced | |
| In case of reproduced technique, report if there were adaptations and what were they | |
| In case of use of substance that promotes cellular alteration, report name, function, concentration, percentage, exposure time | |
| Time period of each step | |
| Temperature (exact 0.0 °C) | |
| Atmosphere conditions (exact 0.0% CO2) | |
| Equipment used | |
| Type of statistical analysis and level of significance | |
| Software for statistical analysis | |