Global ETD Search

91	Mother-child interaction and family functioning : children with cystic fibrosis / Sawyer, Elspeth Henry January 1984 (has links) No description available. Sociology Mother and child Families Cystic fibrosis
92	Adherence of Pseudomonas aeruginosa to perfused tracheal epithelium : adhesin [i.e. adhesion] - receptor interactions / Marcus, Hilda January 1985 (has links) No description available. Biology Pseudomonas aeruginosa Trachea Epithelium Cystic fibrosis
93	The Expression and Characterization of Human Cystic Fibrosis Transmembrane Conductance Regulator (CFTR) in Tobacco Witt, William T. 03 September 2003 (has links) The cystic fibrosis transmembrane conductance regulator (CFTR) is one of the most studied membrane protein models because of its clear clinical significance. Mutations within the CFTR gene lead to cystic fibrosis, the most common autosomal recessive genetic disorder in the Caucasian population. CFTR, a large 160 kDa glycoprotein, is a chloride ion channel in the ABC superfamily of transporter proteins. Due to low natural abundance of CFTR and difficulties producing sufficient amounts in heterologous systems, the exact protein function/structure relationship is unknown. Expression of CFTR in E. coli is lethal and mammalian culture systems are expensive and low yielding. However, successful bioproduction of many complex human proteins has been shown in transgenic plants. Our research objective is to develop tobacco as a model system for expressing human CFTR. Constructs of full-length CFTR fused to the 35S double enhanced promoter could not be propagated in E. coli, suggesting that the CFTR product generated by "leaky" expression was detrimental to bacteria. Two strategies were undertaken to address the problem: 1) a plant intron was introduced into CFTR sequence and 2) a more tightly regulated wound-inducible promoter MeGATM was used. Tobacco was transformed with all constructs. CFTR presence was determined by polymerase chain reaction (PCR). Expression and intron splicing was analyzed by reverse transcriptase-PCR. Splicing did not occur presumably due to intron /exon contexts. In tobacco expressing MeGA:CFTR, however, novel high-molecular-weight membrane-associated proteins were immunodetected using anti-CFTR antibodies suggesting that tobacco may be capable of producing human CFTR. / Master of Science bioproduction tobacco cystic fibrosis transgenic CFTR
94	The role of CFTR in male reproduction and the underlying mechanisms. / CUHK electronic theses & dissertations collection January 2008 (has links) As CFTR plays an important role in HCO3- transport, and HCO3- sensitive soluble adenylyl cyclase (sAC) has been shown to be largely responsible for the cAMP production in spermatogenetic cells, we hypothesized that CFTR-mediated HCO3- transport was important to spermatogenesis via sAC pathway in spermatogenetic and Sertoli cells. Using intracellular pH measurement, we demonstrated that CFTR is involved in HCO3- transport in Sertoli cells. RT-PCR results showed that increased HCO3- concentrations in the culture medium resulted in upregulation of CFTR expression. The results also showed that the intracellular cAMP level in Sertoli cells increased as the extracellular HCO3- concentration increased. HCO3- also caused phosphorylation of the cAMP response element binding (pCREB) proteins transcription factor on serine 133, a modification known to be required by Sertoli cells to support spermatogenesis. This phosphorylation could be inhibited by CFTR inhibitor, further lending support to the notion that CFTR is important for HCO3- transport in Sertoli cells, leading to HCO3- dependent events that are important for spermatogenesis. / CFTR is known to be widely expressed in epithelial cells of male reproductive tracts, but its expression in spermatogenic cells is less well known. We first confirmed the expression of CFTR in spermatogenic cells and mature sperm in rodents. Our study thus focused on the important role of CFTR in the processes related to male fertility including spermatogenesis and sperm capacitation. / Cystic fibrosis transmembrane conductance regulator (CFTR) is an anion channel, mutations of which cause cystic fibrosis, a disease characterized by defective Cl- and HCO3- transport. While over 95% of CF male patients are infertile because of congenital bilateral absence of the vas deferens (CBAVD), the question whether CFTR mutations are involved in other forms of male infertility is under intense debates. / In conclusion, our study has demonstrated the role of CFTR in male reproductive system. We have further elucidated its possible physiological role and the underlying molecular mechanisms. These studies may pave the way for the development of method strategies for diagnosis and treatment of CFTR related infertility in male. / Our study also detected CFTR in both human and mouse sperm. CFTR inhibitor or antibody significantly reduced sperm capacitation, and the associated HCO 3--dependent events including increases in intracellular pH, cAMP production and membrane hyperpolarization. The fertilizing capacity of the sperm obtained from heterozygous CFTR mutant mice is also significantly lower as compared to that of the wild type. These results suggest that CFTR in sperm may be involved in the transport of HCO3- important for sperm capacitation and that CFTR mutations with impaired CFTR function may lead to reduced sperm fertilizing capacity and male infertility other than CBAVD. / We further demonstrated the physiological role of CFTR in spermatogenesis using CFTR knockout mice as an in vivo model. Although TUNNEL staining showed normal percentage of apoptotic cells in seminiferous tubules, Cftr -/- mice had spermatogenetic defects in histology section and fewer number of mature sperm compared with wild type (WT) mice. Consistent with the proposed role of CFTR in spermatogenesis, RT-PCR and Western blot results showed reduced expression of spennatids specific gene, Protamine 1, Protamine 2, and CREM, which have been known to be involved in the process of spermatogenesis, in Cftr-/- mice. / Xu, Wenming. / "January 2008." / Source: Dissertation Abstracts International, Volume: 69-08, Section: B, page: 4506. / Thesis (Ph.D.)--Chinese University of Hong Kong, 2008. / Includes bibliographical references (p. 121-138). / Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Electronic reproduction. [Ann Arbor, MI] : ProQuest Information and Learning, [200-] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Abstract in English and Chinese. / School code: 1307. Cystic fibrosis--Pathophysiology Infertility, Male Cystic Fibrosis--physiopathology Infertility, Male
95	Genetic adaptation by Pseudomonas aeruginosa during chronic cystic fibrosis infections and genetic variation between strains of P. aeruginosa / Smith, Eric Earl. January 2006 (has links) Thesis (Ph. D.)--University of Washington, 2006. / Vita. Includes bibliographical references (leaves 150-153).
96	Expression and functional significance of the cystic fibrosis transmembrance [sic] conductance regulator (CFTR) in human mast cells Déry, René Eugène. January 2009 (has links) Thesis (Ph.D.)--University of Alberta, 2009. / A thesis submitted to the Faculty of Graduate Studies and Research in partial fulfillment of the requirements for the degree of Doctor of Philosophy in Experimental Medicine, Department of Medicine. Title from pdf file main screen (viewed on November 1, 2009). Includes bibliographical references.
97	Teste da medida da diferença de potencial nasal transepitelial Procianoy, Elenara da Fonseca Andrade January 2014 (has links) O teste da diferença de potencial nasal (DPN) é um exame que mede a diferença bioelétrica através do epitélio nasal, a qual resulta do transporte iônico transepitelial dos íons sódio (Na+), pelo canal ENaC (Epitelial Na+ Channel), e cloro (Cl-), pelo canal CFTR(Cystic Fibrosis Transmembrane Conductance Regulator). DPN tem sido utilizada como teste de auxilio diagnóstico em doenças associadas à disfunção do CFTR, como a Fibrose Cística (FC). FC é uma doença genética autossômica recessiva causada por mutações que afetam o funcionamento do canal CFTR (e secundariamente do ENaC) e levam a manifestações em diversos órgãos. Normalmente a dosagem de cloro no suor acima de 60 mEq/L ou a identificação de mutações nos dois alelos confirmam diagnóstico de FC. Porém, existem casos atípicos com exames considerados inconclusivos onde as características eletrofisiológicas decorrentes da disfunção do CFTR devem ser demonstradas para estabelecimento do diagnóstico. A identificação correta destes casos é importante para instituição do tratamento adequado e definição do prognóstico. O objetivo principal deste trabalho foi padronizar a técnica da DPN para sua futura aplicação como ferramenta diagnóstica através da determinação dos seus valores de referência, de sensibilidade, de especificidade e de concordância entre os resultados das duas narinas. Secundariamente, objetivamos analisar as relações entre a presença de função residual do CFTRe a concentração de cloro no suor, fenótipo pancreático, presença de Pseudomonas aeruginosa, função pulmonar e genótipo na amostra de pacientes comFC. Foi realizado um estudo transversal com realização da DPN em um grupo de pacientes com FC (n=29, idade:15±6 anos) e dois grupos controle: não=FC (n=19, idade: 15 ± 10 anos) e sadios (n=19, idade: 17 ± 8 anos). Os resultados demonstraram que os valores da DPN são significativamente diferentes no grupo FC (FC: DPNmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e indiceDPN: 0.85 ± 0.23; não-FC:DPNmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV e indiceDPN: 0.11 ± 0.11) e sadios: DPNmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV e indiceDPN: 0.20±0.14),com sensibilidade e especificidade de 95-96% e concordância de resultado entre as duas narinas maior para a DPNmax (r=0,934). A função residual da CFTR não mostrou relação com nenhum dos parâmetros fenotípicos avaliados. Somente mostrou relação com a gravidade do genótipo. Entretanto, foi observada relação entre os parâmetros que avaliam a hiperfunção do ENaC existente na FC e o fenótipo. Concluímos com este trabalho que foi possível reproduzir e padronizar esta técnica da DPN e demonstrar que o fenótipo da FC está mais relacionado à alteração do transporte do íon sódio através do ENaC do que à presença de função residual da CFTR. / Nasal potential difference test (NPD) is a test that measures the bioelectrical difference across the nasal epithelium, which results from transepithelial ion transport of sodium (Na+), by ENaC channels (Epitelial Na+ Channel) and chloride (Cl-), by CFTR (Cystic Fibrosis Transmembrane Conductance Regulator).NPD has been used as a diagnostic tool in CFTR related disorders, such as Cystic Fibrosis (CF). CF is an autosomal recessive genetic disease caused by mutations that affect the function of the CFTR channel (andsecondarily of the EnaC)and lead to manifestations in various organs. Normally sweat chloride concentration > 60 mEq / L and identification of two CFTR mutations confirm the CF diagnosis. However there are atypical cases with inconclusive sweat chloride or genetic where the electrophysiological characteristics induced by CFTR dysfunction has to be demonstrated for diagnosis. The correct identification of these cases is important for institution of appropriate treatment and definition of prognosis. The objective of this study was to standardize the NPD for its future application as a diagnostic tool through the determination of reference values, sensibility and specificity and agreement of the results between both examined nostrils. Secondarily, we analyzed the relations between residual CFTR function and sweat chloride concentration, pancreatic phenotype, Pseudomonas aeruginosa positivity, pulmonary function and genotype in the sample of CF patients. It was a transversal study where the NPD was measured in a group of CF patients (n = 29, age: 15 ± 6 years) and two control groups: non-CF (n = 19, age: 15 ± 10 years) and healthy (n = 19, age: 17 ± 8 years). The results showed that NPD was significantly different in CF (NPDmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e NPDindex: 0.85 ± 0.23; non-CF: NPDmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV and NPDindex: 0.11 ± 0.11) and healthy: NPDmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV and NPDindex: 0.20±0.14) with sensibility and specificity of 95-96% and agreement between both nostrils greater for NPDmax (r=0.934). The residual CFTR function did not show relation with all phenotypic parameters evaluated. It just showed relation with genotype severity. Indeed it was observed a relation between the parameters that assess the ENaC hyperfunction that occurs in CF and the phenotype. We concluded with this study that was possible to reproduce and to standardize the NPD and to demonstrate that the phenotype is more related to sodium transport alterations through ENaC than to the presence of residual CFTR function. Fibrose cística Mucosa nasal Transporte de íons Nasal potential difference Cystic fibrosis Atypical cystic fibrosis CFTR ENaC
98	Teste da medida da diferença de potencial nasal transepitelial Procianoy, Elenara da Fonseca Andrade January 2014 (has links) O teste da diferença de potencial nasal (DPN) é um exame que mede a diferença bioelétrica através do epitélio nasal, a qual resulta do transporte iônico transepitelial dos íons sódio (Na+), pelo canal ENaC (Epitelial Na+ Channel), e cloro (Cl-), pelo canal CFTR(Cystic Fibrosis Transmembrane Conductance Regulator). DPN tem sido utilizada como teste de auxilio diagnóstico em doenças associadas à disfunção do CFTR, como a Fibrose Cística (FC). FC é uma doença genética autossômica recessiva causada por mutações que afetam o funcionamento do canal CFTR (e secundariamente do ENaC) e levam a manifestações em diversos órgãos. Normalmente a dosagem de cloro no suor acima de 60 mEq/L ou a identificação de mutações nos dois alelos confirmam diagnóstico de FC. Porém, existem casos atípicos com exames considerados inconclusivos onde as características eletrofisiológicas decorrentes da disfunção do CFTR devem ser demonstradas para estabelecimento do diagnóstico. A identificação correta destes casos é importante para instituição do tratamento adequado e definição do prognóstico. O objetivo principal deste trabalho foi padronizar a técnica da DPN para sua futura aplicação como ferramenta diagnóstica através da determinação dos seus valores de referência, de sensibilidade, de especificidade e de concordância entre os resultados das duas narinas. Secundariamente, objetivamos analisar as relações entre a presença de função residual do CFTRe a concentração de cloro no suor, fenótipo pancreático, presença de Pseudomonas aeruginosa, função pulmonar e genótipo na amostra de pacientes comFC. Foi realizado um estudo transversal com realização da DPN em um grupo de pacientes com FC (n=29, idade:15±6 anos) e dois grupos controle: não=FC (n=19, idade: 15 ± 10 anos) e sadios (n=19, idade: 17 ± 8 anos). Os resultados demonstraram que os valores da DPN são significativamente diferentes no grupo FC (FC: DPNmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e indiceDPN: 0.85 ± 0.23; não-FC:DPNmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV e indiceDPN: 0.11 ± 0.11) e sadios: DPNmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV e indiceDPN: 0.20±0.14),com sensibilidade e especificidade de 95-96% e concordância de resultado entre as duas narinas maior para a DPNmax (r=0,934). A função residual da CFTR não mostrou relação com nenhum dos parâmetros fenotípicos avaliados. Somente mostrou relação com a gravidade do genótipo. Entretanto, foi observada relação entre os parâmetros que avaliam a hiperfunção do ENaC existente na FC e o fenótipo. Concluímos com este trabalho que foi possível reproduzir e padronizar esta técnica da DPN e demonstrar que o fenótipo da FC está mais relacionado à alteração do transporte do íon sódio através do ENaC do que à presença de função residual da CFTR. / Nasal potential difference test (NPD) is a test that measures the bioelectrical difference across the nasal epithelium, which results from transepithelial ion transport of sodium (Na+), by ENaC channels (Epitelial Na+ Channel) and chloride (Cl-), by CFTR (Cystic Fibrosis Transmembrane Conductance Regulator).NPD has been used as a diagnostic tool in CFTR related disorders, such as Cystic Fibrosis (CF). CF is an autosomal recessive genetic disease caused by mutations that affect the function of the CFTR channel (andsecondarily of the EnaC)and lead to manifestations in various organs. Normally sweat chloride concentration > 60 mEq / L and identification of two CFTR mutations confirm the CF diagnosis. However there are atypical cases with inconclusive sweat chloride or genetic where the electrophysiological characteristics induced by CFTR dysfunction has to be demonstrated for diagnosis. The correct identification of these cases is important for institution of appropriate treatment and definition of prognosis. The objective of this study was to standardize the NPD for its future application as a diagnostic tool through the determination of reference values, sensibility and specificity and agreement of the results between both examined nostrils. Secondarily, we analyzed the relations between residual CFTR function and sweat chloride concentration, pancreatic phenotype, Pseudomonas aeruginosa positivity, pulmonary function and genotype in the sample of CF patients. It was a transversal study where the NPD was measured in a group of CF patients (n = 29, age: 15 ± 6 years) and two control groups: non-CF (n = 19, age: 15 ± 10 years) and healthy (n = 19, age: 17 ± 8 years). The results showed that NPD was significantly different in CF (NPDmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e NPDindex: 0.85 ± 0.23; non-CF: NPDmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV and NPDindex: 0.11 ± 0.11) and healthy: NPDmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV and NPDindex: 0.20±0.14) with sensibility and specificity of 95-96% and agreement between both nostrils greater for NPDmax (r=0.934). The residual CFTR function did not show relation with all phenotypic parameters evaluated. It just showed relation with genotype severity. Indeed it was observed a relation between the parameters that assess the ENaC hyperfunction that occurs in CF and the phenotype. We concluded with this study that was possible to reproduce and to standardize the NPD and to demonstrate that the phenotype is more related to sodium transport alterations through ENaC than to the presence of residual CFTR function. Fibrose cística Mucosa nasal Transporte de íons Nasal potential difference Cystic fibrosis Atypical cystic fibrosis CFTR ENaC
99	Teste da medida da diferença de potencial nasal transepitelial Procianoy, Elenara da Fonseca Andrade January 2014 (has links) O teste da diferença de potencial nasal (DPN) é um exame que mede a diferença bioelétrica através do epitélio nasal, a qual resulta do transporte iônico transepitelial dos íons sódio (Na+), pelo canal ENaC (Epitelial Na+ Channel), e cloro (Cl-), pelo canal CFTR(Cystic Fibrosis Transmembrane Conductance Regulator). DPN tem sido utilizada como teste de auxilio diagnóstico em doenças associadas à disfunção do CFTR, como a Fibrose Cística (FC). FC é uma doença genética autossômica recessiva causada por mutações que afetam o funcionamento do canal CFTR (e secundariamente do ENaC) e levam a manifestações em diversos órgãos. Normalmente a dosagem de cloro no suor acima de 60 mEq/L ou a identificação de mutações nos dois alelos confirmam diagnóstico de FC. Porém, existem casos atípicos com exames considerados inconclusivos onde as características eletrofisiológicas decorrentes da disfunção do CFTR devem ser demonstradas para estabelecimento do diagnóstico. A identificação correta destes casos é importante para instituição do tratamento adequado e definição do prognóstico. O objetivo principal deste trabalho foi padronizar a técnica da DPN para sua futura aplicação como ferramenta diagnóstica através da determinação dos seus valores de referência, de sensibilidade, de especificidade e de concordância entre os resultados das duas narinas. Secundariamente, objetivamos analisar as relações entre a presença de função residual do CFTRe a concentração de cloro no suor, fenótipo pancreático, presença de Pseudomonas aeruginosa, função pulmonar e genótipo na amostra de pacientes comFC. Foi realizado um estudo transversal com realização da DPN em um grupo de pacientes com FC (n=29, idade:15±6 anos) e dois grupos controle: não=FC (n=19, idade: 15 ± 10 anos) e sadios (n=19, idade: 17 ± 8 anos). Os resultados demonstraram que os valores da DPN são significativamente diferentes no grupo FC (FC: DPNmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e indiceDPN: 0.85 ± 0.23; não-FC:DPNmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV e indiceDPN: 0.11 ± 0.11) e sadios: DPNmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV e indiceDPN: 0.20±0.14),com sensibilidade e especificidade de 95-96% e concordância de resultado entre as duas narinas maior para a DPNmax (r=0,934). A função residual da CFTR não mostrou relação com nenhum dos parâmetros fenotípicos avaliados. Somente mostrou relação com a gravidade do genótipo. Entretanto, foi observada relação entre os parâmetros que avaliam a hiperfunção do ENaC existente na FC e o fenótipo. Concluímos com este trabalho que foi possível reproduzir e padronizar esta técnica da DPN e demonstrar que o fenótipo da FC está mais relacionado à alteração do transporte do íon sódio através do ENaC do que à presença de função residual da CFTR. / Nasal potential difference test (NPD) is a test that measures the bioelectrical difference across the nasal epithelium, which results from transepithelial ion transport of sodium (Na+), by ENaC channels (Epitelial Na+ Channel) and chloride (Cl-), by CFTR (Cystic Fibrosis Transmembrane Conductance Regulator).NPD has been used as a diagnostic tool in CFTR related disorders, such as Cystic Fibrosis (CF). CF is an autosomal recessive genetic disease caused by mutations that affect the function of the CFTR channel (andsecondarily of the EnaC)and lead to manifestations in various organs. Normally sweat chloride concentration > 60 mEq / L and identification of two CFTR mutations confirm the CF diagnosis. However there are atypical cases with inconclusive sweat chloride or genetic where the electrophysiological characteristics induced by CFTR dysfunction has to be demonstrated for diagnosis. The correct identification of these cases is important for institution of appropriate treatment and definition of prognosis. The objective of this study was to standardize the NPD for its future application as a diagnostic tool through the determination of reference values, sensibility and specificity and agreement of the results between both examined nostrils. Secondarily, we analyzed the relations between residual CFTR function and sweat chloride concentration, pancreatic phenotype, Pseudomonas aeruginosa positivity, pulmonary function and genotype in the sample of CF patients. It was a transversal study where the NPD was measured in a group of CF patients (n = 29, age: 15 ± 6 years) and two control groups: non-CF (n = 19, age: 15 ± 10 years) and healthy (n = 19, age: 17 ± 8 years). The results showed that NPD was significantly different in CF (NPDmax: -34 ± 9mV, Δamil: -20 ± 9mV, ΔCl: 4 ± 5mV, Δamilo-iso: -19 ± 9 mV e NPDindex: 0.85 ± 0.23; non-CF: NPDmax: -14 ± 5mV, Δamil: -6 ± 3mV, ΔCl: 17 ± 9mV, Δamilo-iso: -1 ± 4 mV and NPDindex: 0.11 ± 0.11) and healthy: NPDmax: -15 ± 4mV, Δamil: -6 ± 3mV, ΔCl: 11 ± 7mV, Δamilo-iso: -2 ± 4 mV and NPDindex: 0.20±0.14) with sensibility and specificity of 95-96% and agreement between both nostrils greater for NPDmax (r=0.934). The residual CFTR function did not show relation with all phenotypic parameters evaluated. It just showed relation with genotype severity. Indeed it was observed a relation between the parameters that assess the ENaC hyperfunction that occurs in CF and the phenotype. We concluded with this study that was possible to reproduce and to standardize the NPD and to demonstrate that the phenotype is more related to sodium transport alterations through ENaC than to the presence of residual CFTR function. Fibrose cística Mucosa nasal Transporte de íons Nasal potential difference Cystic fibrosis Atypical cystic fibrosis CFTR ENaC
100	Growth Deficiency in Cystic Fibrosis is Observable at Birth and Predictive of Early Pulmonary Function Nelson, Rebecca Joan 02 September 2014 (has links) No description available. Genetics cystic fibrosis birth weight pulmonary function cystic fibrosis related diabetes meconium ileus

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