Your search keyword '"Phillips JA 3rd"' showing total 25 results

1. A molecular basis for variation in clinical severity of isolated growth hormone deficiency type II.

Author

Hamid R, Phillips JA 3rd, Holladay C, Cogan JD, Austin ED, Backeljauw PF, Travers SH, and Patton JG

Subjects

Alleles, Cell Line, DNA analysis, DNA genetics, Exons, Female, Genetic Markers, Genetic Variation, Genotype, Humans, Male, Mutation, Pedigree, Pituitary Gland cytology, Pituitary Gland metabolism, Transcription, Genetic, Dwarfism, Pituitary genetics, Human Growth Hormone genetics

Abstract

Context: Dominant-negative GH1 mutations cause familial isolated growth hormone deficiency type II (IGHD II), which is characterized by GH deficiency, occasional multiple anterior pituitary hormone deficiencies, and anterior pituitary hypoplasia. The basis of the variable expression and progression of IGHD II among relatives who share the same GH1 mutation is poorly understood., Objective: We hypothesized that the cellular ratios of mutant/normal GH1 transcripts would correlate with the severity of the IGHD II phenotype. We determined the relative amounts of mutant and normal GH1 transcripts in cell lines and correlated transcript ratios with severity., Design and Patients: Members of the same IGHD II kindred were genotyped for the GH1 E3+1 G/A mutation by DNA sequencing. Ratios of their 17.5-kDa (mutant)/22-kDa (normal) GH1 transcripts were determined in cultured lymphocytes (CLs), and these ratios were correlated with height sd scores obtained before GH replacement therapy., Results: Ratios of 17.5-/22-kDa GH1 transcripts in CLs from family members with the same IGHD II mutation correlated with differences in their height SD scores., Conclusions: Our findings suggest that expression levels of both the mutant and normal GH1 allele are important in the pathogenesis of IGHD II, that the ratio of mutant/normal transcripts may be a predictive marker of the penetrance and severity of IGHD II, and that CLs may be useful as surrogates to study GH1 transcript expression of subjects whose anterior pituitary cells are not available.

Published

2009

2. Isolated growth hormone deficiency type II caused by a point mutation that alters both splice site strength and splicing enhancer function.

Author

Shariat N, Holladay CD, Cleary RK, Phillips JA 3rd, and Patton JG

Subjects

Cells, Cultured, Child, Preschool, Exons genetics, Female, Humans, Infant, Male, Mutation, Pedigree, RNA Interference, Human Growth Hormone deficiency, Metabolic Diseases genetics, Point Mutation genetics, RNA Splice Sites genetics, RNA Splicing genetics

Abstract

A heterozygous single base mutation in the human growth hormone (GH) gene (GH-1) was identified in a family presenting with isolated GH deficiency type II (IGHD II). Affected individuals have a guanine to adenine transition at the first nucleotide of exon 3 (E3+1 G-->A) that results in exon skipping and production of a dominant-negative 17.5-kDa isoform. We show that the mechanistic basis for exon skipping is due to the unique position of this mutation because it weakens the 3' splice site and simultaneously disrupts a splicing enhancer located within the first seven bases of exon 3. A G-->T mutation at this same position not only affects splicing but also results in a premature stop codon for those transcripts that include exon 3. Thus, mutations that alter the first nucleotide of exon 3 illustrate the various mechanisms by which changes in sequence can cause disease: splice site selection, splicing enhancer function, messenger RNA decay, missense mutations, and nonsense mutations. For IGHD II, only exon skipping leads to production of the dominant-negative isoform, with increasing skipping correlating with increasing disease severity.

Published

2008

3. Rescue of pituitary function in a mouse model of isolated growth hormone deficiency type II by RNA interference.

Author

Shariat N, Ryther RC, Phillips JA 3rd, Robinson IC, and Patton JG

Subjects

Animals, Disease Models, Animal, Dwarfism, Pituitary pathology, Humans, Mice, Mice, Inbred C57BL, Mice, Transgenic, Microscopy, Electron, Pituitary Gland, Anterior pathology, Pituitary Gland, Anterior ultrastructure, Recovery of Function, Dwarfism, Pituitary therapy, Genetic Therapy methods, Human Growth Hormone genetics, Pituitary Gland, Anterior physiology, RNA Interference

Abstract

Splicing mutations in the human GH (hGH) gene (GH-1) that cause skipping of exon 3 result in a form of GH deficiency termed isolated GH deficiency type II (IGHD II). The GH-1 gene contains five exons; constitutive splicing produces the wild-type 22-kDa hormone, whereas skipping of exon 3 results in transcripts encoding a 17.5-kDa isoform that acts as a dominant-negative to block secretion of the wild-type hormone. Common characteristics of IGHD II include short stature due to impaired bone elongation, growth, and, in severe cases, anterior pituitary hypoplasia. Typically, IGHD II is treated by sc delivery of hGH, which can rescue stature but, unfortunately, does not inhibit pituitary hypoplasia. Direct destruction of transcripts encoding the dominant-negative 17.5-kDa isoform should both rescue stature and prevent hypoplasia. Here, we have used delivery of short hairpin RNAs to rescue a murine model of IGHD II by specifically targeting transcripts encoding the 17.5-kDa isoform using RNA interference. To our knowledge, this is the first example where a short hairpin RNA has been expressed to specifically degrade an incorrectly spliced transcript and rescue a dominant-negative disease phenotype in vivo.

Published

2008

4. A case with isolated growth hormone deficiency caused by compound heterozygous mutations in GH-1: a novel missense mutation in the initiation codon and a 7.6kb deletion.

Author

Hayashi Y, Kamijo T, Yamamoto M, Murata Y, Phillips JA 3rd, Ogawa M, and Seo H

Subjects

Alleles, Codon, Initiator genetics, Human Growth Hormone deficiency, Humans, Infant, Male, Methionine chemistry, Methionine genetics, Mutation, Missense, Pedigree, Sequence Analysis, DNA, Valine chemistry, Valine genetics, Dwarfism, Pituitary genetics, Heterozygote, Human Growth Hormone genetics

Abstract

Objective: To characterize the cause of a sporadic isolated growth hormone deficiency in a single patient., Methods: Genomic DNA was extracted from blood samples of the patient and his family. Exons and exon-intron junctions of the GH-1 gene were amplified by PCR and sequenced. To characterize possible GH-1 deletions we performed Southern blot analysis and PCR-restriction fragment length analyses., Results: An adenine to guanine mutation at the first nucleotide of the initiation codon (Met [ATG](-26)Val [GTG]) of the GH-1 gene was identified in the patient and the mother. A 7.6kb GH-1 deletion was identified in the patient, the brother and the father., Conclusion: The patient was a compound heterozygote for an allele bearing a Met(-26)Val missense mutation inherited from his mother and an allele containing deletion of the entire GH-1 gene inherited from his father. The present missense mutation has not been described previously. Attention should be paid to the heterozygous gene deletion that is difficult to detect by PCR-based genetic analysis. The patient responded to GH replacement therapy fairly well, without developing anti-hGH antibody.

Published

2007

5. GH1 gene deletions and IGHD type 1A.

Author

Cogan JD and Phillips JA 3rd

Subjects

Adolescent, Adult, Child, Child Development, Child, Preschool, Dwarfism, Pituitary complications, Dwarfism, Pituitary diagnosis, Dwarfism, Pituitary therapy, Humans, Infant, Infant, Newborn, Middle Aged, Mutation, Dwarfism, Pituitary genetics, Gene Deletion, Human Growth Hormone deficiency, Human Growth Hormone genetics

Abstract

Human Growth Hormone gene ( GH1 ) resides on chromosome 17q22-24 and it is expressed in somatotropic cells of the anterior pituitary gland. While there are multiple causes of GH Deficiency (GHD) a significant proportion have a genetic basis. The most severe Mendelian form of IGHD, called IGHD IA, has an autosomal recessive mode of inheritance. While affected individuals can have short lengths at birth and hypoglycemia in infancy, all develop severe dwarfism by six months of age. Although short stature, delayed growth velocity, and delayed skeletal maturation all occur with IGHD, none are specific for IGHD 1A. GH1 gene deletions, frameshifts, or nonsense mutations cause complete absence of GH in IGHD 1A. Thus IGHD 1A is best described as being complete GHD caused by severe loss of function GH1 gene mutations rather than being limited to only those having GH1 gene deletions. Interestingly, GH1 gene deletions are recurring mutations that can arise through unequal recombination in meiosis rather than by allele sharing through common descent. Individuals with IGHD 1A develop severe dwarfism in early infancy and often develop anti-GH antibodies after receiving exogenous GH. These antibodies can prevent the growth response expected from exogenous GH therapy. Individuals who are heterozygous for a GH1 gene deletion but whose other GH1 allele is not deleted and produces a non truncated product are usually immune tolerant.

Published

2006

6. GH1 splicing is regulated by multiple enhancers whose mutation produces a dominant-negative GH isoform that can be degraded by allele-specific small interfering RNA (siRNA).

Author

Ryther RC, Flynt AS, Harris BD, Phillips JA 3rd, and Patton JG

Subjects

Animals, Base Sequence, Cell Line, Enhancer Elements, Genetic genetics, Exons, Gene Deletion, Humans, Introns, Molecular Sequence Data, Mutation, Protein Isoforms genetics, Alleles, DNA, Recombinant, Enhancer Elements, Genetic physiology, Genes, Dominant, Human Growth Hormone genetics, RNA, Small Interfering physiology

Abstract

The majority of mutations that cause isolated GH deficiency type II affect splicing of GH1 transcripts, leading to the production of a dominant-negative GH isoform. Because numerous mutations and polymorphisms throughout the GH1 gene have not yet been tested for aberrant splicing, we used a deletion mutagenesis screen across intron 2-exon 3-intron 3 to identify splicing regulatory sequences. These analyses identified a new enhancer element, ESE2, upstream of the cryptic splice site in exon 3 and further defined a previously described enhancer (ESE1) to include the first seven nucleotides of exon 3. Besides enhancers, the overall size of intron 3 is also crucial for exon inclusion. Given the deleterious effects of the dominant-negative 17.5-kDa isoform, these and previous studies underscore the extent to which splicing regulatory elements serve to prevent exon skipping. Importantly, we show here that small interfering RNAs can be used to specifically degrade exon 3-skipped transcripts, potentially a new avenue of therapeutic intervention in isolated GH deficiency II and other dominant disorders.

Published

2004

7. Disruption of exon definition produces a dominant-negative growth hormone isoform that causes somatotroph death and IGHD II.

Author

Ryther RC, McGuinness LM, Phillips JA 3rd, Moseley CT, Magoulas CB, Robinson IC, and Patton JG

Subjects

Animals, Base Sequence, DNA Mutational Analysis, Disease Models, Animal, Exons, Humans, Introns, Mice, Mice, Transgenic, Protein Isoforms deficiency, Protein Isoforms genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics, Metabolism, Inborn Errors genetics, Mutation, RNA Splicing

Abstract

Isolated growth hormone deficiency type II (IGHD II) is characterized by short stature due to dominant-negative mutations of the human growth hormone gene (GH1). Most of the known mutations responsible for IGHD II cause aberrant splicing of GH1 transcripts. We have recently shown that mutations that cause exon 3 skipping and produce a dominant-negative 17.5-kDa isoform in humans also cause a dose-dependent disruption of GH secretory vesicles when expressed in GC cells and transgenic mice. We show here that overexpression of the dominant-negative 17.5-kDa isoform also destroys the majority of somatotrophs, leading to anterior pituitary hypoplasia in transgenic mice. It is, therefore, important to understand the regulation of GH1 splicing and why its perturbation causes IGHD II. We demonstrate that dual splicing enhancers are required to ensure exon 3 definition to produce full-length 22-kDa hormone. We also show that splicing enhancer mutations that weaken exon 3 recognition produce variable amounts of the 17.5-kDa isoform, a result which could potentially explain the clinical variability observed in IGHD II. Non-canonical splicing mutations that disrupt splicing enhancers, such as those illustrated here, demonstrate the importance of enhancer elements in regulating alternative splicing to prevent human disease.

Published

2003

8. Novel mutations of the growth hormone 1 (GH1) gene disclosed by modulation of the clinical selection criteria for individuals with short stature.

Author

Millar DS, Lewis MD, Horan M, Newsway V, Easter TE, Gregory JW, Fryklund L, Norin M, Crowne EC, Davies SJ, Edwards P, Kirk J, Waldron K, Smith PJ, Phillips JA 3rd, Scanlon MF, Krawczak M, Cooper DN, and Procter AM

Subjects

Adolescent, Child, Child, Preschool, DNA Mutational Analysis methods, Female, Genetic Variation, Genotype, Growth Disorders etiology, Haplotypes genetics, Human Growth Hormone physiology, Humans, Infant, Male, Mutation, Missense, Phenotype, Promoter Regions, Genetic genetics, Promoter Regions, Genetic physiology, RNA Splicing genetics, RNA Splicing physiology, RNA, Messenger genetics, White People genetics, Growth Disorders genetics, Human Growth Hormone genetics, Patient Selection

Abstract

Subtle mutations in the growth hormone 1 (GH1) gene have been regarded as a comparatively rare cause of short stature. Such lesions were sought in a group of 41 individuals selected for short stature, reduced height velocity, and bone age delay; a group of 11 individuals with short stature and idiopathic growth hormone deficiency (IGHD); and a group of 154 controls. Heterozygous mutations were identified in all three groups but disproportionately in the individuals with short stature, both with (odds ratio 25.2; 95% CI, 5.1-132.2) and without (odds ratio 3.6; 95% CI, 1.0-12.9) IGHD. Twenty-four novel GH1 gene lesions were found. Thirteen novel missense mutations were characterized by assaying the signal transduction activity of in vitro expressed variants; six (T27I, K41R, N47D, S71F, S108R, and T175A) exhibited a reduced ability to activate the JAK/STAT pathway. Molecular modeling suggested that both K41R and T175A might compromise GH receptor binding. Seven GH variants (R16C, K41R, S71F, E74K, Q91L, S108C, and a functional polymorphism, V110I) manifested reduced secretion in rat pituitary cells after allowance had been made for the level of expression attributable to the associated GH1 proximal promoter haplotype. A further leader peptide variant (L-11P) was not secreted. Eleven novel mutations in the GH1 gene promoter were assessed by reporter gene assay but only two, including a GH2 gene-templated gene conversion, were found to be associated with a significantly reduced level of expression. Finally, a novel intron 2 acceptor splice-site mutation, detected in a family with autosomal dominant type II IGHD, was shown to lead to the skipping of exon 3 from the GH1 transcript. A total of 15 novel GH1 gene mutations were thus considered to be of probable phenotypic significance. Such lesions are more prevalent than previously recognized and although most may be insufficient on their own to account for the observed clinical phenotype, they are nevertheless likely to play a contributory role in the etiology of short stature., (Copyright 2003 Wiley-Liss, Inc.)

Published

2003

9. Autosomal dominant growth hormone deficiency disrupts secretory vesicles in vitro and in vivo in transgenic mice.

Author

McGuinness L, Magoulas C, Sesay AK, Mathers K, Carmignac D, Manneville JB, Christian H, Phillips JA 3rd, and Robinson IC

Subjects

Animals, Cell Line, Disease Models, Animal, Female, Gene Expression, Genes, Dominant, Growth Hormone-Releasing Hormone genetics, Human Growth Hormone deficiency, Hypothalamus physiology, In Vitro Techniques, Male, Mice, Mice, Transgenic, Microscopy, Fluorescence, Rats, Transfection, Dwarfism, Pituitary genetics, Dwarfism, Pituitary pathology, Human Growth Hormone genetics, Secretory Vesicles pathology

Abstract

Autosomal dominant GH deficiency type II (IGHDII) is often associated with mutations in the human GH gene (GH1) that give rise to products lacking exon-3 ((Deltaexon3)hGH). In the heterozygous state, these act as dominant negative mutations that prevent the release of human pituitary GH (hGH). To determine the mechanisms of these dominant negative effects, we used a combination of transgenic and morphological approaches in both in vitro and in vivo models. Rat GC cell lines were generated expressing either wild-type GH1 (WT-hGH-GC) or a genomic GH1 sequence containing a G->A transition at the donor splice site of IVS3 ((Deltaexon3)hGH-GC). WT-hGH-GC cells grew normally and produced equivalent amounts of human and rGH packaged in dense-cored secretory vesicles (SVs). In contrast, (Deltaexon3)hGH-GC cells showed few SVs but accumulated secretory product in amorphous cytoplasmic aggregates. They produced much less rGH and grew more slowly than WT-hGH-GC cells. When cotransfected with an enhanced green fluorescent protein construct (GH-eGFP), which copackages with GH in SVs, WT-hGH-GC cells showed normal electron microscopy morphology and SV movements, tracked with total internal reflectance fluorescence microscopy. In contrast, coexpression of (Deltaexon3)hGH with GH-eGFP abolished the vesicular targeting of GH-eGFP, which instead accumulated in static aggregates. Transgenic mice expressing (Deltaexon3)hGH in somatotrophs showed an IGHD-II phenotype with mild to severe pituitary hypoplasia and dwarfism, evident at weaning in the most severely affected lines. Hypothalamic GHRH expression was up-regulated and somatostatin expression reduced in (Deltaexon3)hGH transgenic mice, consistent with their profound GHD. Few SVs were detectable in the residual pituitary somatotrophs in (Deltaexon3)hGH transgenic mice, and these cells showed grossly abnormal morphology. A low copy number transgenic line showed a mild effect relatively specific for GH, whereas two severely affected lines with higher transgene copy numbers showed early onset, widespread pituitary damage, macrophage invasion, and multiple hormone deficiencies. These new in vitro and in vivo models shed new light on the cellular mechanisms involved in IGHDII, as well as its phenotypic consequences in vivo.

Published

2003

10. GH Gene Deletions and IGHD type IA.

Author

Moseley CT, Orenstein MD, and Phillips JA 3rd

Subjects

Dwarfism, Pituitary diagnosis, Dwarfism, Pituitary epidemiology, Dwarfism, Pituitary physiopathology, Frameshift Mutation, Gene Frequency, Human Growth Hormone immunology, Humans, Reverse Transcriptase Polymerase Chain Reaction, Dwarfism, Pituitary genetics, Gene Deletion, Human Growth Hormone genetics

Published

2002

11. Mutations of the GH gene.

Author

Phillips JA 3rd

Subjects

Human Growth Hormone deficiency, Humans, Mutation, RNA, Messenger analysis, Human Growth Hormone genetics

Published

2002

12. An exon splice enhancer mutation causes autosomal dominant GH deficiency.

Author

Moseley CT, Mullis PE, Prince MA, and Phillips JA 3rd

Subjects

Adult, Aged, Alleles, Amino Acid Sequence genetics, DNA Restriction Enzymes, Female, Humans, Infant, Male, Metabolic Diseases genetics, Middle Aged, Molecular Sequence Data, Pedigree, RNA, Messenger genetics, Enhancer Elements, Genetic genetics, Exons genetics, Genes, Dominant, Human Growth Hormone deficiency, Point Mutation physiology, RNA Splicing

Abstract

Familial isolated GH deficiency type II (IGHD II) is caused, in some cases, by heterogeneous IVS3 mutations that affect GH mRNA splicing. We report here our finding an A-->G transition of the fifth base of exon 3 (E3+ 5 A-->G) in affected individuals from an IGHD II family. This mutation disrupts a (GAA)(n) exon splice enhancer (ESE) motif immediately following the weak IVS2 3' splice site. The mutation also destroys an MboII site used to demonstrate heterozygosity in all affected family members. To determine the effect of ESE mutations on GH mRNA processing, GH(3) cells were transfected with expression constructs containing the normal ESE, +5 A-->G, or other ESE mutations, and cDNAs derived from the resulting GH mRNAs were sequenced. All ESE mutations studied reduced activation of the IVS2 3' splice site and caused either partial E3 skipping, due to activation of an E3+ 45 cryptic 3' splice site, or complete E3 skipping. Partial or complete E3 skipping led to loss of the codons for amino acids 32-46 or 32-71, respectively, of the mature GH protein. Our data indicate that the E3+ 5 A-->G mutation causes IGHD II because it perturbs an ESE required for GH splicing.

Published

2002

13. Three new mutations in the gene for the growth hormone (gh)-releasing hormone receptor in familial isolated gh deficiency type ib.

Author

Salvatori R, Fan X, Phillips JA 3rd, Espigares-Martin R, Martin De Lara I, Freeman KL, Plotnick L, Al-Ashwal A, and Levine MA

Subjects

Adolescent, Amino Acid Sequence genetics, Animals, Base Sequence genetics, CHO Cells, Child, Preschool, Cricetinae, Humans, Molecular Sequence Data, Pedigree, Receptors, Neuropeptide metabolism, Receptors, Pituitary Hormone-Regulating Hormone metabolism, Human Growth Hormone deficiency, Mutation genetics, Receptors, Neuropeptide genetics, Receptors, Pituitary Hormone-Regulating Hormone genetics

Abstract

Isolated GH deficiency (IGHD) is familial in 5-30% of cases. The majority of patients have the type IB form, characterized by autosomal recessive transmission, low but measurable serum concentrations of GH, and responsiveness to exogenous GH therapy. Unique mutations in the gene encoding the GHRH receptor (GHRHR) have previously been described in 2 kindreds with IGHD IB. However, the prevalence of GHRHR mutations in patients with IGHD IB is unknown. We analyzed 30 families with IGHD IB in which more than 1 member was affected. Linkage analysis was performed in 28 of the families, and in 3 families sibling pair analysis indicated linkage to the GHRHR gene locus. These 3 families as well as 2 families in which linkage analysis was not performed were screened for mutations in the 13 coding exons, the intron-exon boundaries, and 327 bases of the promoter of the GHRHR gene. We identified novel GHRHR missense mutations in 2 of the 3 kindreds with informative linkage and in 1 family in which linkage had not been performed. In 1 family affected members were homozygous for a mutation in codon 144 that replaces leucine with histidine (L144H). Affected subjects in a second family were compound heterozygotes, carrying both the L144H mutation and a second mutation in codon 242 that replaces phenylalanine with cysteine. Affected subjects in a third family were homozygous for a mutation that replaces alanine at codon 222 with glutamic acid. All 3 mutations segregated with the IGHD phenotype. All 3 mutant receptors were expressed in CHO cells, and each failed to show a cAMP response after treatment of the cells with GHRH. These results demonstrate that missense mutations in the GHRHR gene are a cause of IGHD IB, and that defects in the GHRHR gene may be a more common cause of GH deficiency than previously suspected.

Published

2001

14. Pituitary gene mutations and the growth hormone pathway.

Author

Moseley CT and Phillips JA 3rd

Subjects

Drug Resistance, Dwarfism, Pituitary genetics, Human Growth Hormone physiology, Human Growth Hormone therapeutic use, Humans, Hypopituitarism genetics, Pituitary Hormones deficiency, Receptors, Somatotropin genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics, Mutation, Pituitary Hormones genetics

Abstract

Hereditary forms of pituitary insufficiency not associated with anatomic defects of the central nervous system, hypothalamus, or pituitary are a heterogeneous group of disorders that result from interruptions at different points in the hypothalamic-pituitary-somatomedin-peripheral tissue axis. These different types of pituitary dwarfism can be classified on the level of the defect; mode of inheritance; whether the phenotype is isolated growth hormone deficiency (IGHD) or combined pituitary hormone deficiency (CPHD); whether the hormone is absent, deficient, or abnormal; and, in patients with GH resistance, whether insulin-like growth factor 1 (IGF1) is deficient due to GH receptor or IGF1 defects. Information on each disorder is summarized. More detailed information can be obtained through the electronic database Online Mendelian Inheritance in Man which is available at http://www3.ncbi.nlm.nih.gov/Omim/.

Published

2000

15. Screening for mutations in the GH-1 gene by dideoxy fingerprinting (ddF).

Author

Miyata I, Eto Y, Kamijo T, Ogawa M, Futrakul A, and Phillips JA 3rd

Subjects

Autoradiography, DNA genetics, DNA Fingerprinting, HeLa Cells, Humans, Japan, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction, Thailand, Growth Disorders genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics, Mutation

Published

1999

16. Familial growth hormone deficiency associated with MRI abnormalities.

Author

Hamilton J, Chitayat D, Blaser S, Cohen LE, Phillips JA 3rd, and Daneman D

Subjects

Child, DNA Fingerprinting, Growth Disorders genetics, Human Growth Hormone genetics, Humans, Karyotyping, Magnetic Resonance Imaging, Male, Pituitary Gland, Anterior diagnostic imaging, Pituitary Gland, Posterior diagnostic imaging, Radiography, Growth Disorders diagnostic imaging, Human Growth Hormone deficiency

Abstract

Idiopathic growth hormone deficiency is, in most cases, a sporadic condition. In a number of these patients magnetic resonance imaging (MRI) demonstrates a small anterior pituitary, small or absent pituitary stalk, and ectopically located posterior pituitary. These findings have been attributed to a developmental defect, trauma, or ischemia at birth. We report on a case of familial isolated growth hormone deficiency with mother and son demonstrating the MRI findings described above. The son also had a Chiari type I malformation and medial deviation of the carotid arteries secondary to a narrow skull base. Testing failed to identify a mutation in either the Pit-1 gene or GH gene cluster. This case appears to be an autosomal dominant defect in early development, lending support to the hypothesis that dysgenesis, rather than birth trauma, may cause a small anterior pituitary and ectopic posterior pituitary.

Published

1998

17. Characterization of an intron splice enhancer that regulates alternative splicing of human GH pre-mRNA.

Author

McCarthy EM and Phillips JA 3rd

Subjects

Animals, Base Sequence, Cell Line, Consensus Sequence, DNA genetics, DNA Primers genetics, Exons, Genes, Dominant, Human Growth Hormone deficiency, Humans, In Vitro Techniques, Molecular Sequence Data, Mutagenesis, Site-Directed, Point Mutation, Polymerase Chain Reaction, Rats, Repetitive Sequences, Nucleic Acid, Sequence Deletion, Alternative Splicing genetics, Enhancer Elements, Genetic, Human Growth Hormone genetics, Introns, RNA Precursors genetics, RNA Precursors metabolism

Abstract

Splicing of pre-mRNA transcripts is regulated by consensus sequences at intron (intervening sequence, IVS) boundaries and the branch site. In vitro studies have shown that the small introns of some genes also require intron splice enhancers (ISE) to modulate splice site selection. An autosomal dominant form of isolated GH deficiency (IGHD-II) is caused by mutations in IVS3 of the GH-1 gene that cause exon 3 (E3) skipping, resulting in truncated hGH products that prevent secretion of normal hGH. Interestingly, some of these IGHD-II mutations perturb an ISE that is buried in IVS3. We localized this ISE by quantitating the effects of deletions within IVS3 on E3 skipping. The importance of individual nucleotides to ISE function was determined by analyzing the effects of point mutants and additional deletions. Our results show that (i) an ISE with a G2X1-4G3motif resides in IVS3 of GH-1; (ii) both runs of Gs are required for ISE function; (iii) a single copy of the ISE regulates E3 skipping and (iv) ISE function can be modified by an adjacent AC element. Our findings reveal a new mechanism by which mutations can cause inherited human endocrine disorders and suggest that (i) ISEs may regulate splicing of transcripts of other genes and (ii) mutations of these ISEs or of the trans -acting factors that bind them may cause other genetic disorders.

Published

1998

18. The molecular genetics of growth hormone deficiency.

Author

Procter AM, Phillips JA 3rd, and Cooper DN

Subjects

Base Sequence, Disease Models, Animal, Genetic Diseases, Inborn genetics, Genotype, Human Growth Hormone genetics, Humans, Molecular Sequence Data, Mutation genetics, Phenotype, Receptors, Neuropeptide genetics, Receptors, Pituitary Hormone-Regulating Hormone genetics, Human Growth Hormone deficiency

Abstract

Although most cases of short stature associated with growth hormone (GH) deficiency are sporadic and idiopathic, some 5-30% have an affected first degree relative consistent with a genetic aetiology for the condition. Several different types of mutational lesion in the pituitary-expressed growth hormone (GH1) gene have been described in affected individuals. This review focuses primarily on the GH1 mutational spectrum and its unusual features, discusses potential mechanisms of mutagenesis and pathogenesis, and examines the correlation between mutant genotype and clinical phenotype. The characterization of pathological lesions in several other pituitary-expressed genes that are epistatic to GH1 (POU1F1, PROP1 and GHRHR) has identified additional causes of GH deficiency, the molecular genetics of which are also explored.

Published

1998

19. An improved polymerase chain reaction (PCR) protocol for unambigous detection of growth hormone gene deletions.

Author

Mone CM, Nigro V, Rotondi M, Del Buono A, Mazziotti G, Riondino M, Sinisi AM, Ghizzoni L, Phillips JA 3rd, Bellastella A, and Carella C

Subjects

Ethidium, Fluorescent Dyes, Humans, Gene Deletion, Genetic Carrier Screening, Homozygote, Human Growth Hormone genetics, Polymerase Chain Reaction methods

Abstract

hGH-1 gene deletions are detected by simultaneous PCR amplification along the two homologous DNA sequences flanking the hGH-1 gene on both sides and are differentiated by SmaI restriction enzyme digestion. We have observed that among the SmaI digested PCR products from normal homozygous subjects, from those heterozygous for the 7.6 kb deletion and from those heterozygous for a 6.7 kb deletion, along with the expected fragments there is an unexpected 1470 bp fragment. This fragment arises from the co-amplification of a third homologous sequence located downstream from the hGH-1 gene and it confuses differentiation between normal homozygous and heterozygous for 7.6 kb subjects from the 6.7 kb heterozygous subjects. To overcome this problem we have improved PCR conditions using a different reverse primer. These changes avoid the interaction of the primers with the third homologous sequence located downstream from the hGH-1 gene and prevent the appearance of this additional band that complicates the interpretation of the results. We conclude that the new reverse primer sequence avoids the amplification of the downstream hGH-1 gene sequence and the production of the 1474 bp band after SmaI endonuclease enzyme digestion and makes it possible to differentiate homozygous normal subjects and those who are heterozygous for a 7.6 kb deletion from those who are heterozygous for a 6.7 kb deletion.

Published

1998

20. Clinical and molecular characterization of Brazilian patients with growth hormone gene deletions.

Author

Arnhold IJ, Osorio MG, Oliveira SB, Estefan V, Kamijo T, Krishnamani MR, Cogan JD, Phillips JA 3rd, and Mendonca BB

Subjects

Brazil, Child, Preschool, Female, Growth Disorders diagnosis, Human Growth Hormone therapeutic use, Humans, Infant, Male, Pedigree, Gene Deletion, Growth Disorders genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics

Abstract

Genomic DNA from 23 patients with isolated growth hormone (GH) deficiency (12 males and 11 females: heights -4.9 +/- 1.4 SDS) was screened for GH gene deletions by restriction endonuclease analysis of polymerase chain reaction amplification products. Three unrelated patients had typical features of severe GH deficiency and deletions (6.7 kb in two and 7.6 kb in one) of the GH gene. The two patients with 6.7-kb deletions developed growth-attenuating anti-GH antibodies whereas the patient with the 7.6-kb deletion continued to grow with GH replacement therapy. Our finding that 3/23 (approximately 13%) Brazilian subjects had GH gene deletions agrees with previous studies of severe isolated GH deficiency subjects in other populations. Two of three subjects (67%) with deletions developed blocking antibodies despite administration of exogenous GH at low doses. Interestingly, only 1/10 of cases with affected relatives or parental consanguinity had GH-1 gene deletions.

Published

1998

21. Growth disorders caused by genetic defects in the growth hormone pathway.

Author

Cogan JD and Phillips JA 3rd

Subjects

Growth Disorders metabolism, Growth Hormone-Releasing Hormone metabolism, Human Growth Hormone deficiency, Human Growth Hormone metabolism, Humans, Mutation, Receptors, Neuropeptide metabolism, Receptors, Pituitary Hormone-Regulating Hormone metabolism, Syndrome, Growth Disorders genetics, Human Growth Hormone biosynthesis

Abstract

The growth hormone (GH) pathway is composed of a series of interdependent genes whose products are required for normal growth (Fig 1). The GH pathway genes include ligands (GH and insulin-like growth factor 1 [lGF-1]), transcription factors (prophet of pit 1, or prop 1 and pit 1), agonists and antagonists (growth hormone-releasing hormone [GHRH] and somatostatin), and receptors (GHRH receptor [GHRHR] and the GH receptor [GHR]). These genes are expressed in different organs and tissues, including the hypothalamus, pituitary, liver, and bone. Effective and regulated expression of the growth hormone pathway is essential for growth in stature as well as homeostasis of carbohydrate, protein, and fat metabolism.

Published

1998

22. Allelic variations in the human growth hormone-1 gene promoter of growth hormone-deficient patients and normal controls.

Author

Wagner JK, Eblé A, Cogan JD, Prince MA, Phillips JA 3rd, and Mullis PE

Subjects

Base Sequence, Humans, Molecular Sequence Data, Pedigree, Reference Values, Alleles, Genetic Variation genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics, Promoter Regions, Genetic genetics

Abstract

Objective: Isolated growth hormone deficiency (IGHD) type IB is suggested to be more probably due to alterations in the genes directly involved in the hypothalamo-pituitary axis and/or in the specific transcriptional regulation (cis-trans coupling) of the hGH-1 gene than to alterations in the gene itself. In this study we analyzed the hGH-1 gene promoter region for structural alterations and allelic variations., Methods: The hGH-1 gene promoter region was analyzed by PCR, cycle sequencing and direct-blotting electrophoresis in a total of 212 individuals including 113 patients with IGHD type IB, 21 unaffected family members and 78 normal controls., Results: Twenty-two sequence variation sites were identified. Of these, 14% were located around the region of -1075bp, 77% between -550bp and the translational start site (+1bp) and 9% within the first intron. Only one variation site affected a characterized cis-acting element, namely that of NF-1. Importantly, all the variations found in patients were also observed in non-affected family members as well as in normal unrelated controls., Conclusions: These findings imply that it is not a single variation within the GH-1 gene promoter, and therefore in the cis-acting elements, which causes IGHD. However, we can not exclude the possibility that combinations of variations might perturb expression. Furthermore, these data illustrate the normal heterogeneity of the GH-1 gene promoter region, a fact that has to be borne in mind whenever transcriptional studies are performed.

Published

1997

23. A novel mechanism of aberrant pre-mRNA splicing in humans.

Author

Cogan JD, Prince MA, Lekhakula S, Bundey S, Futrakul A, McCarthy EM, and Phillips JA 3rd

Subjects

Alleles, Base Sequence, Child, Preschool, DNA, Deoxyribonucleases, Type II Site-Specific metabolism, HeLa Cells, Humans, Molecular Sequence Data, Mutation, Human Growth Hormone deficiency, Human Growth Hormone genetics, RNA Precursors, RNA Splicing

Abstract

Eukaryotic pre-mRNA splicing is regulated by consensus sequences at the intron boundaries and branch site. Recently, Sirand-Pugnet et al. reported the importance of an additional intronic sequence, an (A/U)GGG repeat in chicken beta-tropomyosin that is a binding site for a protein required for spliceosome assembly. Interestingly, we have detected mutations in IVS3 of the human growth hormone (GH) gene that affect a putative, homologous consensus sequence and which also perturb splicing. In a series of dominant-negative GH mutations that cause exon skipping, we found two mutations that do not occur within the 5' and 3' splice sites, or branch consensus sites. The first mutation is a G-->A transition of the 28th base (+28G-->A) of and the second deletes 18 bp (del+28-45) of IVS3 of the human GH gene. These mutations segregated with autosomal dominant GH deficiency in both kindreds and no other allelic GH gene changes were detected. RT-PCR amplification of transcripts from expression vectors containing the +28G-->A or del+28-45 alleles yielded products showing a >10-fold preferred use of alternative splicing, similar to findings previously reported for IVS3 donor site mutations. Both mutations are located 28 bp downstream from the 5' splice site and examination of the sequences perturbed revealed an intronic XGGG repeat similar to the repeat found to regulate mRNA splicing in chicken beta-tropomyosin. Interestingly, the XGGG repeats involved in our mutations exhibit homologous spacing to those in a so-called 'winner' RNA sequence. Binding of A1 heterogeneous nuclear ribonucleoprotein (hnRNP) by 'winner' sequences in pre-mRNA transcripts is thought to play an important role in pre-mRNA packaging and transport as well as 5' splice site selection in pre-mRNAs that contain multiple 5' splice sites. Our findings suggest that (i) XGGG repeats may regulate alternative splicing in the human GH gene and (ii) mutations of these repeats cause GH deficiency by perturbing alternative splicing. Mutations of homologous intron sequences may underlie other human diseases.

Published

1997

24. Detection of growth hormone gene defects by dideoxy fingerprinting (ddF).

Author

Miyata I, Cogan JD, Prince MA, Kamijo T, Ogawa M, and Phillips JA 3rd

Subjects

Autoradiography, Base Sequence, DNA Primers chemistry, Humans, Japan, Polymerase Chain Reaction, Reference Values, Sequence Analysis, DNA, DNA Fingerprinting, Growth Disorders genetics, Human Growth Hormone deficiency, Human Growth Hormone genetics, Mutation genetics

Abstract

We carried out screening for mutations in the GH-1 gene in 29 sporadic Japanese subjects with severe Isolated Growth Hormone Deficiency (IGHD) by dideoxy fingerprinting (ddF). Three of 29 (approximately 10%) were heterozygous for each of the following GH-1 gene mutations including: 1) an G-->A transition in the third codon of the GH-1 signal peptide of exon 1 resulting in a Threonine to Alanine substitution, 2) a G-->A transition in the first base of the donor splice site of IVS 3 (+1G-->A) and 3) a G-->A transition in the 183rd codon of the GH-1 mature peptide of exon 5 resulting in an Arginine to Histidine substitution. One of three was heterozygous for both mutations of 1) and 2). The IVS 3 (+1G-->A) mutation has been previously reported in affected individuals from three unrelated families with IGHD type II (autosomal dominant form). This mutation destroys the GH IVS 3 donor splice site, causing skipping of exon 3 and loss of the codons for amino acids 32-71 of the mature GH peptide. Our findings indicate that 1) ddF screening of genomic DNAs provides a practical tool to detect GH gene mutations and 2) some sporadic cases of IGHD may be caused by GH gene alternations.

Published

1997

25. An improved polymerase chain reaction (PCR) protocol for unambigous detection of growth hormone gene deletions

Author

Vincenzo Nigro, A.M. Sinisi, Gherardo Mazziotti, C. M. Mone, John A. Phillips, Mario Rotondi, A. Del Buono, Carlo Carella, M. Riondino, L. Ghizzoni, Antonio Bellastella, Mone, Cm, Nigro, Vincenzo, Rotondi, M, DEL BUONO, A, Mazziotti, G, Riondino, M, Sinisi, Am, Ghizzoni, L, PHILLIPS JA, 3rd, Bellastella, A, and Carella, C.

Subjects

Endocrinology, Diabetes and Metabolism, Genetic Carrier Screening, Polymerase Chain Reaction, DNA sequencing, SmaI, law.invention, Endonuclease, Endocrinology, law, Ethidium, Homologous chromosome, Medicine, Humans, Gene, Polymerase chain reaction, Fluorescent Dyes, Genetics, biology, business.industry, Human Growth Hormone, Homozygote, Molecular biology, Pediatrics, Perinatology and Child Health, biology.protein, business, Nested polymerase chain reaction, Gene Deletion

Abstract

hGH-1 gene deletions are detected by simultaneous PCR amplification along the two homologous DNA sequences flanking the hGH-1 gene on both sides and are differentiated by SmaI restriction enzyme digestion. We have observed that among the SmaI digested PCR products from normal homozygous subjects, from those heterozygous for the 7.6 kb deletion and from those heterozygous for a 6.7 kb deletion, along with the expected fragments there is an unexpected 1470 bp fragment. This fragment arises from the co-amplification of a third homologous sequence located downstream from the hGH-1 gene and it confuses differentiation between normal homozygous and heterozygous for 7.6 kb subjects from the 6.7 kb heterozygous subjects. To overcome this problem we have improved PCR conditions using a different reverse primer. These changes avoid the interaction of the primers with the third homologous sequence located downstream from the hGH-1 gene and prevent the appearance of this additional band that complicates the interpretation of the results. We conclude that the new reverse primer sequence avoids the amplification of the downstream hGH-1 gene sequence and the production of the 1474 bp band after SmaI endonuclease enzyme digestion and makes it possible to differentiate homozygous normal subjects and those who are heterozygous for a 7.6 kb deletion from those who are heterozygous for a 6.7 kb deletion.

Published

1998