The Caenorhabditis elegans K10C2.4 Gene Encodes a Member of the Fumarylacetoacetate Hydrolase Family

Fisher, Alfred L.; Page, Kathryn; Lithgow, Gordon J.; Nash, Lindsey

doi:10.1074/jbc.m708341200

Cited by 35 publications

(75 citation statements)

References 55 publications

(67 reference statements)

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“…The HGO, an enzyme upstream of FAH in the Tyr degradation pathway, is essential for the catalysis of homogentisate into MAA and FAA (Lindblad et al, 1977). Inactivation of HGO in fungi, mice, and worms, therefore, was able to rescue the lethality associated with FAH mutations (Fernández-Cañón and Peñalva, 1995b;Manning et al, 1999;Fisher et al, 2008). Through generation of the double mutant sscd1 hgo, we also found that disruption of the Arabidopsis putative HGO is able to completely eliminate the spontaneous cell death in the sscd1 mutant (Fig.…”

Section: Discussionmentioning

confidence: 63%

“…In both human HT1 and mouse fah mutants, the metabolic intermediates (MAA, FAA, succinylacetoacetate, and succinylacetone) were highly accumulated, which are toxic to cells and tissues (Lindblad et al, 1977;Grompe et al, 1993;Aponte et al, 2001;Jorquera and Tanguay, 2001). Due to technical difficulties, it is so far not possible to detect these metabolic intermediates in entire worms (Fisher et al, 2008) and in Arabidopsis plants (data not shown). To verify that the cell death phenotype in the sscd1 mutant might also have resulted from the accumulation of succinylacetoacetate and succinylacetone, we followed the approach used in worms (Fisher et al, 2008) and treated Arabidopsis seedlings with succinylacetone, the unique product that is commercially available among these metabolic intermediates.…”

Section: Succinylacetone Induces Cell Death In Arabidopsismentioning

confidence: 99%

“…Due to technical difficulties, it is so far not possible to detect these metabolic intermediates in entire worms (Fisher et al, 2008) and in Arabidopsis plants (data not shown). To verify that the cell death phenotype in the sscd1 mutant might also have resulted from the accumulation of succinylacetoacetate and succinylacetone, we followed the approach used in worms (Fisher et al, 2008) and treated Arabidopsis seedlings with succinylacetone, the unique product that is commercially available among these metabolic intermediates. We found that treatment of wild-type seedlings with succinylacetone mimicked the sscd1 phenotypes: the treated wild-type seedlings exhibited wilted leaves and slow-growth symptoms under LD (Fig.…”

Section: Succinylacetone Induces Cell Death In Arabidopsismentioning

confidence: 99%

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Disruption of Fumarylacetoacetate Hydrolase Causes Spontaneous Cell Death under Short-Day Conditions in Arabidopsis

et al. 2013

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Fumarylacetoacetate hydrolase (FAH) hydrolyzes fumarylacetoacetate to fumarate and acetoacetate, the final step in the tyrosine (Tyr) degradation pathway that is essential to animals. Deficiency of FAH in animals results in an inborn lethal disorder. However, the role for the Tyr degradation pathway in plants remains to be elucidated. In this study, we isolated an Arabidopsis (Arabidopsis thaliana) short-day sensitive cell death1 (sscd1) mutant that displays a spontaneous cell death phenotype under short-day conditions. The SSCD1 gene was cloned via a map-based cloning approach and found to encode an Arabidopsis putative FAH. The spontaneous cell death phenotype of the sscd1 mutant was completely eliminated by further knockout of the gene encoding the putative homogentisate dioxygenase, which catalyzes homogentisate into maleylacetoacetate (the antepenultimate step) in the Tyr degradation pathway. Furthermore, treatment of Arabidopsis wild-type seedlings with succinylacetone, an abnormal metabolite caused by loss of FAH in the Tyr degradation pathway, mimicked the sscd1 cell death phenotype. These results demonstrate that disruption of FAH leads to cell death in Arabidopsis and suggest that the Tyr degradation pathway is essential for plant survival under short-day conditions.

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Section: Discussionmentioning

confidence: 63%

Section: Succinylacetone Induces Cell Death In Arabidopsismentioning

confidence: 99%

Section: Succinylacetone Induces Cell Death In Arabidopsismentioning

confidence: 99%

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Disruption of Fumarylacetoacetate Hydrolase Causes Spontaneous Cell Death under Short-Day Conditions in Arabidopsis

et al. 2013

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“…This can lead to the construction of a transgene which is more reflective of the native expression pattern, or the construction of a functional transgene when other approaches fail 5 . The resulting transgenes can carry a variety of epitope tags including GFP or a TAP tag.…”

Section: Discussionmentioning

confidence: 99%

“…While these transgenes are often successful with regards to producing a GFP reporter gene or expressing a cDNA in a desired pattern, these transgenes can lack the alternate promoters, enhancer elements, and 3' untranslated region (UTR) elements which play important roles in the control of gene expression in vivo 2 . For example, both the daf-12 and fah-1 genes have important enhancer elements which lie outside of the proximal promoter which were missed in promoter only constructs 3,4,5 . Further many transgene constructs use the unc-54 3'UTR which prevents regulation by the appropriate microRNA genes 6,7,8 .…”

Section: Overviewmentioning

confidence: 99%

The Production of <em>C. elegans</em> Transgenes via Recombineering with the <em>galK</em> Selectable Marker

Zhang

Kashyap

Ferguson

et al. 2011

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The creation of transgenic animals is widely utilized in C. elegans research including the use of GFP fusion proteins to study the regulation and expression pattern of genes of interest or generation of tandem affinity purification (TAP) tagged versions of specific genes to facilitate their purification. Typically transgenes are generated by placing a promoter upstream of a GFP reporter gene or cDNA of interest, and this often produces a representative expression pattern. However, critical elements of gene regulation, such as control elements in the 3' untranslated region or alternative promoters, could be missed by this approach. Further only a single splice variant can be usually studied by this means. In contrast, the use of worm genomic DNA carried by fosmid DNA clones likely includes most if not all elements involved in gene regulation in vivo which permits the greater ability to capture the genuine expression pattern and timing. To facilitate the generation of transgenes using fosmid DNA, we describe an E. coli based recombineering procedure to insert GFP, a TAP-tag, or other sequences of interest into any location in the gene. The procedure uses the galK gene as the selection marker for both the positive and negative selection steps in recombineering which results in obtaining the desired modification with high efficiency. Further, plasmids containing the galK gene flanked by homology arms to commonly used GFP and TAP fusion genes are available which reduce the cost of oligos by 50% when generating a GFP or TAP fusion protein. These plasmids use the R6K replication origin which precludes the need for extensive PCR product purification. Finally, we also demonstrate a technique to integrate the unc-119 marker on to the fosmid backbone which allows the fosmid to be directly injected or bombarded into worms to generate transgenic animals. This video demonstrates the procedures involved in generating a transgene via recombineering using this method. Protocol OverviewMany transgenes used in the generation of transgenic C. elegans consist of promoter sequences and perhaps a gene cDNA cloned into one of the vectors generated by the lab of Dr. Andy Fire 1 . While these transgenes are often successful with regards to producing a GFP reporter gene or expressing a cDNA in a desired pattern, these transgenes can lack the alternate promoters, enhancer elements, and 3' untranslated region (UTR) elements which play important roles in the control of gene expression in vivo 2 . For example, both the daf-12 and fah-1 genes have important enhancer elements which lie outside of the proximal promoter which were missed in promoter only constructs 3,4,5 . Further many transgene constructs use the unc-54 3'UTR which prevents regulation by the appropriate microRNA genes 6,7,8 . Consequently, generating transgenes with large segments of worm genomic DNA would be ideal for capturing all of promoters, splice variants, and 3' UTR control elements. Recently a C. elegans fosmid library which consists of~40 kb regions of genomic ...

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Phenylalanine hydroxylase: Function, structure, and regulation

2013

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Mammalian phenylalanine hydroxylase (PAH) catalyzes the rate-limiting step in the phenylalanine catabolism, consuming about 75% of the phenylalanine input from the diet and protein catabolism under physiological conditions. In humans, mutations in the PAH gene lead to phenylketonuria (PKU), and most mutations are mainly associated with PAH misfolding and instability. The established treatment for PKU is a phenylalanine-restricted diet and, recently, supplementation with preparations of the natural tetrahydrobiopterin cofactor also shows effectiveness for some patients. Since 1997 there has been a significant increase in the understanding of the structure, catalytic mechanism, and regulation of PAH by its substrate and cofactor, in addition to improved correlations between genotype and phenotype in PKU. Importantly, there has also been an increased number of studies on the structure and function of PAH from bacteria and lower eukaryote organisms, revealing an additional anabolic role of the enzyme in the synthesis of melanin-like pigments. In this review, we discuss these recent studies, which contribute to define the evolutionary adaptation of the PAH structure and function leading to sophisticated regulation for effective catabolic processing of phenylalanine in mammalian organisms. V C 2013 IUBMB Life, 65(4): [341][342][343][344][345][346][347][348][349] 2013

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The Caenorhabditis elegans K10C2.4 Gene Encodes a Member of the Fumarylacetoacetate Hydrolase Family

Cited by 35 publications

References 55 publications

Disruption of Fumarylacetoacetate Hydrolase Causes Spontaneous Cell Death under Short-Day Conditions in Arabidopsis

Disruption of Fumarylacetoacetate Hydrolase Causes Spontaneous Cell Death under Short-Day Conditions in Arabidopsis

The Production of <em>C. elegans</em> Transgenes via Recombineering with the <em>galK</em> Selectable Marker

Phenylalanine hydroxylase: Function, structure, and regulation

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