Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing

Detalhes bibliográficos
Autor(a) principal: Ferrara, Taise Fernanda da Silva [UNIFESP]
Data de Publicação: 2018
Tipo de documento: Tese
Idioma: por
Título da fonte: Repositório Institucional da UNIFESP
Texto Completo: https://sucupira.capes.gov.br/sucupira/public/consultas/coleta/trabalhoConclusao/viewTrabalhoConclusao.jsf?popup=true&id_trabalho=6513887
https://repositorio.unifesp.br/handle/11600/53043
Resumo: Huanglongbing (HLB or citrus greening) is a bacterial disease that affects the citrus crop and nowadays represent the greatest threat to the world's citrus industry. HLB is associated with the phloemlimited bacterium Candidatus Liberibacter asiaticus (CLas) that is transmitted by the vector insect Diaphorina citri. D. citri psyllid belongs to the hemiptera order and has in its digestive tract enzymes of the class of cysteine peptidases as the most abundant proteolytic enzymes, being able to be involved in different processes of development in the insect. In this context, the aim of this work was the identification, cloning, recombinant expression, enzymatic characterization and gene expression analysis of two cysteine peptidases such as cathepsin Blike (DCcatB2) and a cathepsin Llike (DCcatL1) of insect D. citri. The recombinant proteins expressed in Rosetta E. coli cells (DE3) were solubilized in ureacontaining buffer, purified by affinity chromatography and renatured by the refolding process. The enzyme DCcatL1 was activated at pH 4.5 and presented higher activity at 37°C. The catalytic activity was determined using the fluorogenic substrates ZFRAMC and ZLRAMC. DCcatL1 presented higher affinity by ZFRAMC with a Km of 12.29 μM and a kcat/Km = 63 M1s1 and was efficiently inhibited by E64 and by four citrus recombinant cystatins (CclemCPI1, CclemCPI2, CsinCPI1 and CsinCPI2). The cystatin CsinCPI2 showed higher inhibitory potency against DCcatL1 with a Ki = 4.46 pM. The analysis of DCcatL1 gene expression showed high expression in the gut of D. citri, being 2.59 times higher than in head and 2.87 times than in carcass. In the developmental phases, DCcatL1 was more expressed in egg, than in nymph and adult, suggesting a nondigestive and therefore a lysosomal role for this enzyme. The enzyme DCcatB2 was activated at pH 4.0 exhibiting higher affinity for the ZFRAMC substrate (Km = 42.97 μM) when compared to ZRRAMC (Km = 78.9 μM). The activity of DCcatB2 was strongly inhibited by the cathepsin B specific inhibitor CA074 and by the cystatin CclemCPI1 with a Ki of 12 nM and 7.6 nM, respectively. The analysis of the gene expression of DCcatB2 in the developmental phases of D. citri showed a high expression in egg, when compared to nymph and adult. In the body parts of D. citri, DCcatB2 was 6.8 times more expressed in carcass and 5.2 times in head when compared to the gut, suggesting a nondigestive and non lysosomal role for this enzyme. Our results point DCcatL1 and DCcatB2 as promising targets for the development of a control strategy against HLB.
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spelling Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros HuanglongbingIdentification and characterization of targets for control the insect Diaphorina citri, vector of the citrus Huanglongbing diseaseHuanglongbingCathepsinsCystinsDiaphorina citriHuanglongbingCitrosCatepsinasCistatinasHuanglongbing (HLB or citrus greening) is a bacterial disease that affects the citrus crop and nowadays represent the greatest threat to the world's citrus industry. HLB is associated with the phloemlimited bacterium Candidatus Liberibacter asiaticus (CLas) that is transmitted by the vector insect Diaphorina citri. D. citri psyllid belongs to the hemiptera order and has in its digestive tract enzymes of the class of cysteine peptidases as the most abundant proteolytic enzymes, being able to be involved in different processes of development in the insect. In this context, the aim of this work was the identification, cloning, recombinant expression, enzymatic characterization and gene expression analysis of two cysteine peptidases such as cathepsin Blike (DCcatB2) and a cathepsin Llike (DCcatL1) of insect D. citri. The recombinant proteins expressed in Rosetta E. coli cells (DE3) were solubilized in ureacontaining buffer, purified by affinity chromatography and renatured by the refolding process. The enzyme DCcatL1 was activated at pH 4.5 and presented higher activity at 37°C. The catalytic activity was determined using the fluorogenic substrates ZFRAMC and ZLRAMC. DCcatL1 presented higher affinity by ZFRAMC with a Km of 12.29 μM and a kcat/Km = 63 M1s1 and was efficiently inhibited by E64 and by four citrus recombinant cystatins (CclemCPI1, CclemCPI2, CsinCPI1 and CsinCPI2). The cystatin CsinCPI2 showed higher inhibitory potency against DCcatL1 with a Ki = 4.46 pM. The analysis of DCcatL1 gene expression showed high expression in the gut of D. citri, being 2.59 times higher than in head and 2.87 times than in carcass. In the developmental phases, DCcatL1 was more expressed in egg, than in nymph and adult, suggesting a nondigestive and therefore a lysosomal role for this enzyme. The enzyme DCcatB2 was activated at pH 4.0 exhibiting higher affinity for the ZFRAMC substrate (Km = 42.97 μM) when compared to ZRRAMC (Km = 78.9 μM). The activity of DCcatB2 was strongly inhibited by the cathepsin B specific inhibitor CA074 and by the cystatin CclemCPI1 with a Ki of 12 nM and 7.6 nM, respectively. The analysis of the gene expression of DCcatB2 in the developmental phases of D. citri showed a high expression in egg, when compared to nymph and adult. In the body parts of D. citri, DCcatB2 was 6.8 times more expressed in carcass and 5.2 times in head when compared to the gut, suggesting a nondigestive and non lysosomal role for this enzyme. Our results point DCcatL1 and DCcatB2 as promising targets for the development of a control strategy against HLB.A doença bacteriana Huanglongbing (HLB ou greening) que afeta a cultura dos citros é hoje considerada a maior ameaça à indústria cítrica mundial. O HLB está associado à presença da bactéria Candidatus Liberibacter asiaticus (CLas) no floema das plantas e é transmitida pelo inseto vetor Diaphorina citri. O psilídeo D. citri pertence à ordem hemíptera e possui em seu trato digestivo as enzimas da classe das cisteíno peptidases como as enzimas proteolíticas mais abundantes, podendo estas estar envolvidas em diferentes processos de desenvolvimento no inseto. Nesse contexto, os objetivos deste trabalho foram a identificação, clonagem, expressão recombinante, caracterização enzimática e análise da expressão gênica de duas cisteíno peptidases do tipo catepsina B (DCcatB2) e uma catepsina L (DCcatL1) de D. citri. As proteínas recombinantes expressas em células de E.coli Rosetta (DE3) foram solubilizadas em tampão contendo uréia, purificadas por cromatografia de afinidade e renaturadas pelo processo de refolding. A enzima DCcatL1 foi ativada em pH 4,5 e apresentou maior atividade a 37°C. A atividade catalítica foi determinada utilizando os substratos fluorogênicos ZFRMCA e ZLRMCA. DCcatL1 apresentou maior afinidade por ZFRMCA com um Km de 12,29 μM e um kcat/Km = 63 M1s1 e foi eficientemente inibida por E64 e por quatro cistatinas recombinantes de citros (CclemCPI1, CclemCPI2, CsinCPI1 e CsinCPI2). A cistatina CsinCPI2 apresentou maior potência inibitória contra DCcatL1 com um Ki = 4,46 pM. A análise da expressão gênica de DCcatL1 mostrou elevada expressão no intestino de D. citri, sendo 2,59 vezes mais alta do que em cabeça e 2,87 vezes do que em carcaça. Nas fases de desenvolvimento, DCcatL1 foi mais expressa em ovo, do que em ninfa e adulto, sugerindo um papel não digestivo e portanto lisossomal para esta enzima. A enzima DCcatB2 foi ativada em pH 4,0 apresentando maior afinidade pelo substrato ZFRMCA (Km = 42,97 μM) quando comparado ao ZRRMCA (Km = 78,9 μM). A atividade de DCcatB2 foi fortemente inibida pelo inibidor específico de catepsina B CA074 e pela cistatina cClemCPI1 com Ki de 12 nM e 7,6 nM, respectivamente. A análise da expressão gênica de DCcatB2 nas fases de desenvolvimento de D. citri mostrou elevada expressão em ovo, quando comparada a ninfa e adulto. Nas partes do corpo de D. citri, DCcatB2 foi 6,8 vezes mais expressa em carcaça e 5,2 vezes em cabeça quando comparadas ao intestino, sugerindo um papel não digestivo e não lisossomal para a enzima. Nossos resultados apontam DCcatL1 e DCcatB2 como alvos promissores para o desenvolvimento de uma estratégia de controle contra o HLB.Dados abertos - Sucupira - Teses e dissertações (2018)Universidade Federal de São Paulo (UNIFESP)Carmona, Adriana Karaoglanovic [UNIFESP]Fuentes, Andrea Soares da Costahttp://lattes.cnpq.br/2426157257540389http://lattes.cnpq.br/2122863342403909http://lattes.cnpq.br/1515264534466259Universidade Federal de São Paulo (UNIFESP)Ferrara, Taise Fernanda da Silva [UNIFESP]2020-03-25T12:10:52Z2020-03-25T12:10:52Z2018-11-28info:eu-repo/semantics/doctoralThesisinfo:eu-repo/semantics/publishedVersion100 f.application/pdfhttps://sucupira.capes.gov.br/sucupira/public/consultas/coleta/trabalhoConclusao/viewTrabalhoConclusao.jsf?popup=true&id_trabalho=65138872018-0988.pdfhttps://repositorio.unifesp.br/handle/11600/53043porSão Pauloinfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UNIFESPinstname:Universidade Federal de São Paulo (UNIFESP)instacron:UNIFESP2024-08-02T20:18:04Zoai:repositorio.unifesp.br/:11600/53043Repositório InstitucionalPUBhttp://www.repositorio.unifesp.br/oai/requestbiblioteca.csp@unifesp.bropendoar:34652024-08-02T20:18:04Repositório Institucional da UNIFESP - Universidade Federal de São Paulo (UNIFESP)false
dc.title.none.fl_str_mv Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
Identification and characterization of targets for control the insect Diaphorina citri, vector of the citrus Huanglongbing disease
title Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
spellingShingle Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
Ferrara, Taise Fernanda da Silva [UNIFESP]
Huanglongbing
Cathepsins
Cystins
Diaphorina citri
Huanglongbing
Citros
Catepsinas
Cistatinas
title_short Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
title_full Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
title_fullStr Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
title_full_unstemmed Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
title_sort Identificação e caracterização de alvos para controle do inseto Diaphorina citri, vetor da doença do citros Huanglongbing
author Ferrara, Taise Fernanda da Silva [UNIFESP]
author_facet Ferrara, Taise Fernanda da Silva [UNIFESP]
author_role author
dc.contributor.none.fl_str_mv Carmona, Adriana Karaoglanovic [UNIFESP]
Fuentes, Andrea Soares da Costa
http://lattes.cnpq.br/2426157257540389
http://lattes.cnpq.br/2122863342403909
http://lattes.cnpq.br/1515264534466259
Universidade Federal de São Paulo (UNIFESP)
dc.contributor.author.fl_str_mv Ferrara, Taise Fernanda da Silva [UNIFESP]
dc.subject.por.fl_str_mv Huanglongbing
Cathepsins
Cystins
Diaphorina citri
Huanglongbing
Citros
Catepsinas
Cistatinas
topic Huanglongbing
Cathepsins
Cystins
Diaphorina citri
Huanglongbing
Citros
Catepsinas
Cistatinas
description Huanglongbing (HLB or citrus greening) is a bacterial disease that affects the citrus crop and nowadays represent the greatest threat to the world's citrus industry. HLB is associated with the phloemlimited bacterium Candidatus Liberibacter asiaticus (CLas) that is transmitted by the vector insect Diaphorina citri. D. citri psyllid belongs to the hemiptera order and has in its digestive tract enzymes of the class of cysteine peptidases as the most abundant proteolytic enzymes, being able to be involved in different processes of development in the insect. In this context, the aim of this work was the identification, cloning, recombinant expression, enzymatic characterization and gene expression analysis of two cysteine peptidases such as cathepsin Blike (DCcatB2) and a cathepsin Llike (DCcatL1) of insect D. citri. The recombinant proteins expressed in Rosetta E. coli cells (DE3) were solubilized in ureacontaining buffer, purified by affinity chromatography and renatured by the refolding process. The enzyme DCcatL1 was activated at pH 4.5 and presented higher activity at 37°C. The catalytic activity was determined using the fluorogenic substrates ZFRAMC and ZLRAMC. DCcatL1 presented higher affinity by ZFRAMC with a Km of 12.29 μM and a kcat/Km = 63 M1s1 and was efficiently inhibited by E64 and by four citrus recombinant cystatins (CclemCPI1, CclemCPI2, CsinCPI1 and CsinCPI2). The cystatin CsinCPI2 showed higher inhibitory potency against DCcatL1 with a Ki = 4.46 pM. The analysis of DCcatL1 gene expression showed high expression in the gut of D. citri, being 2.59 times higher than in head and 2.87 times than in carcass. In the developmental phases, DCcatL1 was more expressed in egg, than in nymph and adult, suggesting a nondigestive and therefore a lysosomal role for this enzyme. The enzyme DCcatB2 was activated at pH 4.0 exhibiting higher affinity for the ZFRAMC substrate (Km = 42.97 μM) when compared to ZRRAMC (Km = 78.9 μM). The activity of DCcatB2 was strongly inhibited by the cathepsin B specific inhibitor CA074 and by the cystatin CclemCPI1 with a Ki of 12 nM and 7.6 nM, respectively. The analysis of the gene expression of DCcatB2 in the developmental phases of D. citri showed a high expression in egg, when compared to nymph and adult. In the body parts of D. citri, DCcatB2 was 6.8 times more expressed in carcass and 5.2 times in head when compared to the gut, suggesting a nondigestive and non lysosomal role for this enzyme. Our results point DCcatL1 and DCcatB2 as promising targets for the development of a control strategy against HLB.
publishDate 2018
dc.date.none.fl_str_mv 2018-11-28
2020-03-25T12:10:52Z
2020-03-25T12:10:52Z
dc.type.driver.fl_str_mv info:eu-repo/semantics/doctoralThesis
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format doctoralThesis
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2018-0988.pdf
https://repositorio.unifesp.br/handle/11600/53043
url https://sucupira.capes.gov.br/sucupira/public/consultas/coleta/trabalhoConclusao/viewTrabalhoConclusao.jsf?popup=true&id_trabalho=6513887
https://repositorio.unifesp.br/handle/11600/53043
identifier_str_mv 2018-0988.pdf
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dc.coverage.none.fl_str_mv São Paulo
dc.publisher.none.fl_str_mv Universidade Federal de São Paulo (UNIFESP)
publisher.none.fl_str_mv Universidade Federal de São Paulo (UNIFESP)
dc.source.none.fl_str_mv reponame:Repositório Institucional da UNIFESP
instname:Universidade Federal de São Paulo (UNIFESP)
instacron:UNIFESP
instname_str Universidade Federal de São Paulo (UNIFESP)
instacron_str UNIFESP
institution UNIFESP
reponame_str Repositório Institucional da UNIFESP
collection Repositório Institucional da UNIFESP
repository.name.fl_str_mv Repositório Institucional da UNIFESP - Universidade Federal de São Paulo (UNIFESP)
repository.mail.fl_str_mv biblioteca.csp@unifesp.br
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