Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada

Detalhes bibliográficos
Ano de defesa: 2013
Autor(a) principal: Mariana de Oliveira Almeida
Orientador(a): Não Informado pela instituição
Banca de defesa: Não Informado pela instituição
Tipo de documento: Dissertação
Tipo de acesso: Acesso aberto
Idioma: por
Instituição de defesa: Universidade Federal de Minas Gerais
Programa de Pós-Graduação: Não Informado pela instituição
Departamento: Não Informado pela instituição
País: Não Informado pela instituição
Palavras-chave em Português:
Hipertensão
Cromatografia líquida
Medicamentos Análise
Espectrometria de massa
Farmácia
Link de acesso: https://hdl.handle.net/1843/EMCO-97GNL6
Resumo: The treatment of hypertension with a single drug is efficient for only one-third of the patients. In order to maximize the efficacy of the treatment, drugs that act in different pathophysiological mechanisms are associated. The combination of olmesartan medoxomil and amlodipine besylate, an angiotensin II type 1 receptor antagonist and calcium channel blocker, respectively, in fixed dose combination tablets is effective, safe and well tolerated. Because it is a new association that is still protected by a patent, there are few articles in the scientific literature that described analytical and bioanalytical methods for the simultaneous quantification of these drugs. An analytical method by high performance liquid chromatography (HPLC) with ultraviolet detection was developed and validated for simultaneous quantification of amlodipine and olmesartan medoxomil in fixed dose combination. The chromatographic analysis was performed in a C18 column, mobile phase composed of acetonitrile:methanol:0.3% triethylamine (30:30:40) pH 2.75 and a flow rate of 1.0 mL/min. Injection volume was 10 µL, detection was at ë 238 nm and run time was 5.5 minutes. Then, the analytical method was transferred to ultra performance liquid chromatography (UPLC) with ultraviolet detection using mathematical formulas to calculate the new injection volume and new flow rate of mobile phase, which were 0.7 µL and 0.613 mL/min., respectively. Adjustments in the solvent composition of mobile phase were performed to improve the efficiency of the UPLC method. The optimized mobile phase was composed of acetonitrile:methanol:0.3% triethylamine (26:26:52) pH 2.75. At this condition, the run time was 1.25 minutes, which provided a reduction of approximately 77% in the analysis time and 86% in solvent consumption. After the method optimization by UPLC, the method was validated. The HPLC method showed to be statistically equivalent to the UPLC method after analysis of three batches of the product BenicarAnlo®. Thus, both methods may be used to perform quality control of olmesartan medoxomil and amlodipine in fixed dose combination tablets. A bioanalytical method was also developed and validated by HPLC with tandem mass spectrometry detection and electrospray ionization in the positive mode for quantifying amlodipine and olmesartan in human plasma. Felodipine and valsartan were used as internal standards of amlodipine and olmesartan, respectively. The sample preparation was carried out using the technique of liquid-liquid extraction. The chromatographic analysis was performed in a C18 column, mobile phase composed of methanol:0.05% formic acid (75:25) and a flow rate of 1.0 mL/min. The transitions employed for the quantification of amlodipine, olmesartan, felodipine and valsartan were m/z 409.4 237.7, m/z 447.6 206.8, m/z 384.7 338.2, m/z 436.5 291.0, respectively. The bioanalytical method showed to be selective, precise, accurate and linear over the range of 1 to 100 ng/mL for amlodipine and 3 to 1800 ng/mL for olmesartan. Therefore, it may be applied in future studies of therapeutic drug monitoring and bioequivalence.
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spelling 2019-08-14T22:27:42Z2025-09-09T00:12:27Z2019-08-14T22:27:42Z2013-02-22https://hdl.handle.net/1843/EMCO-97GNL6The treatment of hypertension with a single drug is efficient for only one-third of the patients. In order to maximize the efficacy of the treatment, drugs that act in different pathophysiological mechanisms are associated. The combination of olmesartan medoxomil and amlodipine besylate, an angiotensin II type 1 receptor antagonist and calcium channel blocker, respectively, in fixed dose combination tablets is effective, safe and well tolerated. Because it is a new association that is still protected by a patent, there are few articles in the scientific literature that described analytical and bioanalytical methods for the simultaneous quantification of these drugs. An analytical method by high performance liquid chromatography (HPLC) with ultraviolet detection was developed and validated for simultaneous quantification of amlodipine and olmesartan medoxomil in fixed dose combination. The chromatographic analysis was performed in a C18 column, mobile phase composed of acetonitrile:methanol:0.3% triethylamine (30:30:40) pH 2.75 and a flow rate of 1.0 mL/min. Injection volume was 10 µL, detection was at ë 238 nm and run time was 5.5 minutes. Then, the analytical method was transferred to ultra performance liquid chromatography (UPLC) with ultraviolet detection using mathematical formulas to calculate the new injection volume and new flow rate of mobile phase, which were 0.7 µL and 0.613 mL/min., respectively. Adjustments in the solvent composition of mobile phase were performed to improve the efficiency of the UPLC method. The optimized mobile phase was composed of acetonitrile:methanol:0.3% triethylamine (26:26:52) pH 2.75. At this condition, the run time was 1.25 minutes, which provided a reduction of approximately 77% in the analysis time and 86% in solvent consumption. After the method optimization by UPLC, the method was validated. The HPLC method showed to be statistically equivalent to the UPLC method after analysis of three batches of the product BenicarAnlo®. Thus, both methods may be used to perform quality control of olmesartan medoxomil and amlodipine in fixed dose combination tablets. A bioanalytical method was also developed and validated by HPLC with tandem mass spectrometry detection and electrospray ionization in the positive mode for quantifying amlodipine and olmesartan in human plasma. Felodipine and valsartan were used as internal standards of amlodipine and olmesartan, respectively. The sample preparation was carried out using the technique of liquid-liquid extraction. The chromatographic analysis was performed in a C18 column, mobile phase composed of methanol:0.05% formic acid (75:25) and a flow rate of 1.0 mL/min. The transitions employed for the quantification of amlodipine, olmesartan, felodipine and valsartan were m/z 409.4 237.7, m/z 447.6 206.8, m/z 384.7 338.2, m/z 436.5 291.0, respectively. The bioanalytical method showed to be selective, precise, accurate and linear over the range of 1 to 100 ng/mL for amlodipine and 3 to 1800 ng/mL for olmesartan. Therefore, it may be applied in future studies of therapeutic drug monitoring and bioequivalence.Universidade Federal de Minas GeraisCromatografia líquida de ultra eficiênciaOlmesartanaCromatografia líquida de alta eficiênciaHipertensãoEspectrometria de massas sequencialOlmesartana medoxomilaAnlodipinoHipertensãoCromatografia líquidaMedicamentos AnáliseEspectrometria de massaFarmáciaDesenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinadainfo:eu-repo/semantics/publishedVersioninfo:eu-repo/semantics/masterThesisMariana de Oliveira Almeidainfo:eu-repo/semantics/openAccessporreponame:Repositório Institucional da UFMGinstname:Universidade Federal de Minas Gerais (UFMG)instacron:UFMGGerson Antonio PianettiIsabela da Costa CesarLeonardo de Souza TeixeiraJacqueline de SouzaO tratamento da hipertensão com apenas um fármaco é eficiente, somente, para um terço dos pacientes. Para maximizar a eficácia do tratamento, associam-se fármacos que atuam em diferentes mecanismos fisiopatológicos. A associação de olmesartana medoxomila e besilato de anlodipino, um antagonista do receptor AT1 de angiotensina II e um bloqueador dos canais de cálcio, respectivamente, em comprimidos de dose fixa combinada é efetiva, segura e bem tolerada. Por ser uma associação nova e que ainda está protegida por patente, há na literatura científica poucos artigos que descreveram métodos analíticos e bioanalíticos para quantificação simultânea desses fármacos. Um método analítico por cromatografia líquida de alta eficiência (CLAE) com detecção por ultravioleta foi desenvolvido e validado para quantificação simultânea de anlodipino e olmesartana medoxomila em dose fixa combinada. A análise cromatográfica foi realizada em coluna C18, a fase móvel foi composta de acetonitrila:metanol:trietilamina 0,3% (30:30:40) pH 2,75 com fluxo de 1,0 mL/min. O volume de injeção foi de 10 µL, a detecção foi em ë 238 nm e o tempo de corrida foi 5,5 minutos. Na sequência, o método foi transferido para cromatografia líquida de ultra eficiência (CLUE) com detecção por ultravioleta com auxílio de fórmulas matemáticas para calcular o novo volume de injeção e novo fluxo da fase móvel, que foram 0,7 ìL e 0,613 mL/min., respectivamente. Ajustes na proporção dos solventes da fase móvel foram realizados para melhorar a eficiência do método por CLUE. A fase móvel otimizada foi composta por acetonitrila:metanol:trietilamina 0,3% (26:26:48) pH 2,75. Nessa condição o tempo de corrida foi 1,25 minutos, o que proporcionou uma redução de aproximadamente 77% no tempo de análise e de 86% no consumo de solvente. Após a otimização do método por CLUE, o método foi validado. Os métodos por CLAE e CLUE demonstraram ser estatisticamente equivalentes após a análise de três lotes do medicamento BenicarAnlo®. Assim, ambos os métodos podem ser utilizados para proceder ao controle de qualidade de anlodipino e olmesartana medoxomila em comprimidos de dose fixa combinada. Um método bioanalítico também foi desenvolvido e validado por CLAE com detecção por espectrometria de massas sequencial e ionização por electrospray no modo positivo para quantificar anlodipino e olmesartana em plasma humano. Felodipino e valsartana foram empregados como padrões internos de anlodipino e olmesartana, respectivamente. O preparo das amostras foi feito por meio da técnica de extração líquido-líquido. A análise cromatográfica foi realizada em coluna C18, com fase móvel composta de metanol:ácido fórmico 0,05% (75:25) a 1,0 mL/min. As transições empregadas para anlodipino, olmesartana, felodipino e valsartana foram m/z 409,4 237,7, m/z 447,6 206,8, m/z 384,7 338,2, m/z 436,5 291,0, respectivamente. O método bioanalítico foi seletivo, preciso, exato e linear na faixa de 1 a 100 ng/mL para anlodipino e de 3 a 1800 ng/mL para olmesartana. Por isso, poderá ser aplicado em estudos futuros de monitorização terapêutica e de bioequivalência.UFMGORIGINALdisserta__o_mestrado_mariana_impress_o.pdfapplication/pdf2727807https://repositorio.ufmg.br//bitstreams/2bf1fdd8-621c-4703-bac7-5520582c5414/download9e3227867844a08fef0c3872ee1833b9MD51trueAnonymousREADTEXTdisserta__o_mestrado_mariana_impress_o.pdf.txttext/plain324630https://repositorio.ufmg.br//bitstreams/82e96807-cfb2-460f-a7ee-42ae1f6c0a43/download484b56c9f37aa371e37fd90f2eaacf48MD52falseAnonymousREADTHUMBNAILdisserta__o_mestrado_mariana_impress_o.pdf.jpgdisserta__o_mestrado_mariana_impress_o.pdf.jpgGenerated Thumbnailimage/jpeg2820https://repositorio.ufmg.br//bitstreams/40b167a4-95ae-4fe4-9078-ddbc35a91440/downloadf4172aa758d8b21950ca410bd4c6d9c8MD53falseAnonymousREAD1843/EMCO-97GNL62025-09-09 15:52:24.169open.accessoai:repositorio.ufmg.br:1843/EMCO-97GNL6https://repositorio.ufmg.br/Repositório InstitucionalPUBhttps://repositorio.ufmg.br/oairepositorio@ufmg.bropendoar:2025-09-09T18:52:24Repositório Institucional da UFMG - Universidade Federal de Minas Gerais (UFMG)false
dc.title.none.fl_str_mv Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
title Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
spellingShingle Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
Mariana de Oliveira Almeida
Hipertensão
Cromatografia líquida
Medicamentos Análise
Espectrometria de massa
Farmácia
Cromatografia líquida de ultra eficiência
Olmesartana
Cromatografia líquida de alta eficiência
Hipertensão
Espectrometria de massas sequencial
Olmesartana medoxomila
Anlodipino
title_short Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
title_full Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
title_fullStr Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
title_full_unstemmed Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
title_sort Desenvolvimento e validação de métodos analíticos e bioanalíticos para os fármacos anlodipino e olmesartana medoxomila, em dose fixa combinada
author Mariana de Oliveira Almeida
author_facet Mariana de Oliveira Almeida
author_role author
dc.contributor.author.fl_str_mv Mariana de Oliveira Almeida
dc.subject.por.fl_str_mv Hipertensão
Cromatografia líquida
Medicamentos Análise
Espectrometria de massa
Farmácia
topic Hipertensão
Cromatografia líquida
Medicamentos Análise
Espectrometria de massa
Farmácia
Cromatografia líquida de ultra eficiência
Olmesartana
Cromatografia líquida de alta eficiência
Hipertensão
Espectrometria de massas sequencial
Olmesartana medoxomila
Anlodipino
dc.subject.other.none.fl_str_mv Cromatografia líquida de ultra eficiência
Olmesartana
Cromatografia líquida de alta eficiência
Hipertensão
Espectrometria de massas sequencial
Olmesartana medoxomila
Anlodipino
description The treatment of hypertension with a single drug is efficient for only one-third of the patients. In order to maximize the efficacy of the treatment, drugs that act in different pathophysiological mechanisms are associated. The combination of olmesartan medoxomil and amlodipine besylate, an angiotensin II type 1 receptor antagonist and calcium channel blocker, respectively, in fixed dose combination tablets is effective, safe and well tolerated. Because it is a new association that is still protected by a patent, there are few articles in the scientific literature that described analytical and bioanalytical methods for the simultaneous quantification of these drugs. An analytical method by high performance liquid chromatography (HPLC) with ultraviolet detection was developed and validated for simultaneous quantification of amlodipine and olmesartan medoxomil in fixed dose combination. The chromatographic analysis was performed in a C18 column, mobile phase composed of acetonitrile:methanol:0.3% triethylamine (30:30:40) pH 2.75 and a flow rate of 1.0 mL/min. Injection volume was 10 µL, detection was at ë 238 nm and run time was 5.5 minutes. Then, the analytical method was transferred to ultra performance liquid chromatography (UPLC) with ultraviolet detection using mathematical formulas to calculate the new injection volume and new flow rate of mobile phase, which were 0.7 µL and 0.613 mL/min., respectively. Adjustments in the solvent composition of mobile phase were performed to improve the efficiency of the UPLC method. The optimized mobile phase was composed of acetonitrile:methanol:0.3% triethylamine (26:26:52) pH 2.75. At this condition, the run time was 1.25 minutes, which provided a reduction of approximately 77% in the analysis time and 86% in solvent consumption. After the method optimization by UPLC, the method was validated. The HPLC method showed to be statistically equivalent to the UPLC method after analysis of three batches of the product BenicarAnlo®. Thus, both methods may be used to perform quality control of olmesartan medoxomil and amlodipine in fixed dose combination tablets. A bioanalytical method was also developed and validated by HPLC with tandem mass spectrometry detection and electrospray ionization in the positive mode for quantifying amlodipine and olmesartan in human plasma. Felodipine and valsartan were used as internal standards of amlodipine and olmesartan, respectively. The sample preparation was carried out using the technique of liquid-liquid extraction. The chromatographic analysis was performed in a C18 column, mobile phase composed of methanol:0.05% formic acid (75:25) and a flow rate of 1.0 mL/min. The transitions employed for the quantification of amlodipine, olmesartan, felodipine and valsartan were m/z 409.4 237.7, m/z 447.6 206.8, m/z 384.7 338.2, m/z 436.5 291.0, respectively. The bioanalytical method showed to be selective, precise, accurate and linear over the range of 1 to 100 ng/mL for amlodipine and 3 to 1800 ng/mL for olmesartan. Therefore, it may be applied in future studies of therapeutic drug monitoring and bioequivalence.
publishDate 2013
dc.date.issued.fl_str_mv 2013-02-22
dc.date.accessioned.fl_str_mv 2019-08-14T22:27:42Z
2025-09-09T00:12:27Z
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