Inborn errors of carbohydrate metabolism

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Inborn errors of carbohydrate metabolism
Specialty Medical genetics
Metabolism of common monosaccharides and related reactions (Carbohydrate Metabolism) Metabolism of common monosaccharides, and related reactions.png
Metabolism of common monosaccharides and related reactions (Carbohydrate Metabolism)

Inborn errors of carbohydrate metabolism are inborn error of metabolism that affect the catabolism and anabolism of carbohydrates.

Contents

An example is lactose intolerance.

Carbohydrates account for a major portion of the human diet. These carbohydrates are composed of three principal monosaccharides: glucose, fructose and galactose; in addition glycogen is the storage form of carbohydrates in humans. The failure to effectively use these molecules accounts for the majority of the inborn errors of human carbohydrates metabolism.

By Carbohydrate

Glycogen and Glucose

Glycogen storage diseases are deficiencies of enzymes or transport proteins which impair glycogen synthesis, glycogen degradation or glycolysis. The two organs most commonly affected are the liver and the skeletal muscle. Glycogen storage diseases that affect the liver typically cause hepatomegaly and hypoglycemia; those that affect skeletal muscle cause exercise intolerance, progressive weakness and cramping. [1]

Glucose-6-phosphate isomerase deficiency affects step 2 of glycolysis. Triosephosphate isomerase deficiency affects step 5 of glycolysis. Phosphoglycerate kinase deficiency affects step 7 of glycolysis. Pyruvate kinase deficiency affects the 10th and last step of glycolysis.

Glucose-6-phosphate dehydrogenase deficiency affects the degradation of glucose in the pentose phosphate pathway, which is especially important in red blood cells.

For further information on inborn errors of glucose metabolism and inborn errors of glycogen metabolism see below.

Lactose

Lactose is a disaccharide sugar composed of galactose and glucose that is found in milk. Lactose can not be absorbed by the intestine and needs to be split in the small intestine into galactose and glucose by the enzyme called lactase; unabsorbed lactose can cause abdominal pain, bloating, diarrhea, gas, and nausea.

In most mammals, production of lactase diminishes after infants are weaned from maternal milk. However, 5% to 90% of the human population possess an advantageous autosomal mutation in which lactase production persists after infancy. The geographic distribution of lactase persistence is concordant with areas of high milk intake. Lactase non-persistence is common in tropical and subtropical countries. Individuals with lactase non-persistency may experience nausea, bloating and diarrhea after ingesting dairy.

Galactose

Galactosemia, the inability to metabolize galactose in liver cells, is the most common monogenic disorder of carbohydrate metabolism, affecting 1 in every 55,000 newborns.[ citation needed ] When galactose in the body is not broken down, it accumulates in tissues. The most common signs are failure to thrive, hepatic insufficiency, cataracts and developmental delay. Long term disabilities include poor growth, mental retardation, and ovarian failure in females. [2]

Galactosemia is caused by mutations in the gene that makes the enzyme galactose-1-phosphate uridylyltransferase. Approximately 70% of galactosemia-causing alleles have a single missense mutation in exon 6. A milder form of galactosemia, called Galactokinase deficiency, is caused a lack of the enzyme uridine diphosphate galactose-4-epimerase which breaks down a byproduct of galactose. This type of is associated with cataracts, but does not cause growth failure, mental retardation, or hepatic disease. Dietary reduction of galactose is also the treatment but not as severe as in patients with classical galactosemia. This deficiency can be systemic or limited to red blood cells and leukocytes.

Screening is performed by measuring GAL-1-P urydil transferase activity. Early identification affords prompt treatment, which consists largely of eliminating dietary galactose.

Fructose

Fructose malabsorption is a digestive disorder in which absorption of fructose is impaired by deficient fructose carriers in the small intestine's enterocytes.

Three autosomal recessive disorders impair fructose metabolism in liver cells. The most common is caused by mutations in the gene encoding hepatic fructokinase, an enzyme that catalyzes the first step in the metabolism of dietary fructose. Inactivation of the hepatic fructokinase results in asymptomatic fructosuria.

Hereditary fructose intolerance (HFI) results in poor feeding, failure to thrive, chronic liver disease and chronic kidney disease, and death. HFI is caused by a deficiency of fructose 1,6-biphosphate aldolase in the liver, kidney cortex and small intestine. Infants and adults are asymptomatic unless they ingest fructose or sucrose.

Deficiency of hepatic fructose 1,6-biphosphate (FBPase) causes impaired gluconeogenesis, hypoglycemia and severe metabolic acidemia. If patients are adequately supported beyond childhood, growth and development appear to be normal.

Essential fructosuria is a clinically benign condition characterized by the incomplete metabolism of fructose in the liver, leading to its excretion in urine.

By affected system

This is a dynamic list and may never be able to satisfy particular standards for completeness. You can help by adding missing items with reliable sources.

Glucose metabolism

Glycolysis

The metabolic pathway glycolysis is used by cells to break down carbohydrates like glucose (and various other simple sugars) in order to extract energy from them. During glycolysis ATP, NADH (both an energy transport form used inside cells) as well as pyruvate are produced.

Glycolysis is taking place in the cytosol where, under anaerobic conditions, pyruvate is converted to lactate. Under aerobic conditions, the pyruvate is transported from the cytosol to the mitochondrion, where further energy can be extracted through the citric acid cycle (CAC) (see below, c.f. bioenergetic systems).

The liver can also create glucose (gluconeogenesis, see below); during times of low carbohydrate supply from the digestive system, the liver creates glucose and supplies it to other organs. [3] Most enzymes of glycolysis also participate in gluconeogenesis, as it is mostly the reverse metabolic pathway of glycolysis; a deficiency of these liver enzymes will therefore impact both glycolysis and gluconeogenesis. (Note: gluconeogenesis is taking place only in the liver and not in other cells like e.g. muscle cells.)

Glycolytic  step
Enzyme 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Management and treatment References
and links
Glycolysis step 1
Glucokinase 		GCK:
Pancreatic beta cells
Hyperinsulinemic hypoglycemia, familial, 3
(HHF3, hyperinsulinism due to glucokinase deficiency) 		Hypoglycemia due to hyperinsulinemia. NLM/GHR:GCK
OMIM: GCK
OMIM: HHF3
GARD: HHF3
ORPHA: HHF3
Glycolysis step 1
Glucokinase 		GCK:
Pancreatic beta cells
Maturity onset diabetes of the young type II
(MODY2, GCK-MODY) 		Diabetes. Hyperglycemia due to hypoinsulinemia while fasting but some glucose tolerance when consuming carbohydrates. NLM/GHR:GCK
OMIM: GCK
OMIM: MODY2
GARD: MODY2
ORPHA: MODY2
Glycolysis step 2
Glucose-6-phosphate isomerase 		GPI:
RBCs
Glucose-6-phosphate isomerase deficiency
(GPI deficiency, GPID, hemolytic anemia due to glucophosphate isomerase deficiency) 		Hemolytic anemia. NLM/GHR:GPI
OMIM: GPI
NLM/GHR:GPID
OMIM: GPID
ORPHA: GPID
Glycolysis step 3
Phosphofructo-kinase 1
(Not involved in glyconeogenesis) 		PFKM:
Muscle, also RBCs
PFKL:
Liver, also RBCs
GSD type VII
(GSD 7, Tarui's Disease,
Phosphofructokinase deficiency) 		Classic form: Symptoms usually appear in early childhood. Myopathy. Exercise-induced muscle cramps, weakness and sometimes rhabdomyolysis. Nausea and vomiting following strenuous exercise. Myoglobinuria, haemolytic anaemia, Hyperuricemia is common. High levels of bilirubin and jaundiced appearance possible.
Late-onset form: Presents later in life. Myopathy, weakness and fatigue. Exercise intolerance (more than in GSD 5). Severe symptoms from classic type are absent.
Infantile form: Rare. Often floppy infant syndrome (hypotonia), arthrogryposis, encephalopathy, cardiomyopathy and respiratory issues. Also central nervous system manifest possible, usually seizures.
Hemolytic form: The defining characteristic is hemolytic anemia. Myopathy not as common.
Rhabdomyolysis/myoglobinuria may cause acute renal failure. 		Exercise test: Late about 3 times increase of lactate (higher than in GSD 5 and lower than in healthy). Increased rise of ammonia. [4] No specific treatment. General advice is avoidance of vigorous exercise and of high-carbohydrate meals. NLM/GHR:PFKM
OMIM: PFKM
OMIM: PFKL
NLM/GHR:GSD VII
OMIM: GSD VII
GARD: GSD VII
ORPHA: GSD VII
Glycolysis step 4
Aldolase A 		ALDOA:
Muscle, also liver and RBCs
GSD type XII
(GSD 12, Aldolase A deficiency, ALDOA deficiency, red cell aldolase deficiency) 		Muscle Symptoms: Myopathy. Exercise intolerance, cramps. In some rhabdomyolysis and myoglobinuria.
Liver Symptoms: In some Hepatomegaly
RBC Symptoms: Hemolytic anemia.
Rhabdomyolysis/myoglobinuria may cause acute renal failure. 		Exercise test: ? No treatment information in references given. NLM/GHR:ALDOA
OMIM: ALDOA
OMIM: GSD XII
GARD: GSD XII
ORPHA: GSD XII
Glycolysis step 4
Aldolase B 		ALDOB:
Liver
Hereditary fructose intolerance
(Aldolase B deficiency, ALDOB deficiency) 		Hypoglycemia. Hepatic and renal dysfunction. NLM/GHR:ALDOB
OMIM: ALDOB
NLM/GHR:ALDOB D
OMIM: ALDOB D
GARD: ALDOB D
ORPHA: ALDOB D
Glycolysis step 4
Aldolase C 		ALDOC:
Brain
Unclear role in: 		Neurodegeneration, unclear role. See respective conditions See respective conditions OMIM: ALDOC
Glycolysis step 5
Triosephosphate isomerase 		TPI1:
RBCs
Triosephosphate isomerase deficiency (TPID) 		Hemolytic anemia. Reticulocytosis and hyperbilirubinemia are common.
Classical generalized form: Progressive neurologic dysfunction with dystonia, tremor, dyskinesia, pyramidal tract signs, cardiomyopathy and spinal motor neuron involvement with progressive neuromuscular impairment (severe weakness and muscle wasting). 		NLM/GHR:TPI1
OMIM: TPI1
NLM/GHR:TPID
OMIM: TPID
GARD: TPID
ORPHA: TPID
Glycolysis step 6
Glyceraldehyde 3-phosphate dehydrogenase 		GAPDH:
Brain
Unclear role in: 		Neurodegeneration, unclear role. See respective conditions See respective conditions OMIM: GAPDH
Glycolysis step 7
Phosphoglycerate kinase 		PGK1:
Muscle, RBCs
Phosphoglycerate kinase deficiency
(PGK1D, PGK deficiency, GSD due to phosphoglycerate kinase 1 deficiency) 		Myopathic form: Progressive muscle weakness, pain, and cramping, particularly with exercise. Myoglobinuria possible.
Myoglobinuria may cause acute renal failure.
Hemolytic form: Hemolytic anemia.
Neurologic form: In some central nervous system manifestation, including hemiplegic migraines, epilepsy, ataxia and tremor. Progressive neurologic impairment in some.
Combinations of 1, 2 or all 3 forms have been reported. 		Exercise test: ? Regular blood transfusions for severe chronic anemia; splenectomy has been shown to be beneficial in some cases. NLM/GHR:PGK1
OMIM: PGK1
NLM/GHR:PGK1D
OMIM: PGK1D
GARD: PGK1D
ORPHA: PGK1D
Glycolysis step 8
Phosphoglycerate mutase 		PGAM2:
Muscle
GSD type X
(GSD 10, muscle phosphoglycerate mutase deficiency, myopathy due to PGAM deficiency, PGAMD) 		Myopathy, exercise intolerance. Exercise-induced cramps, myoglobinuria and myalgia. Rhabdomyolysis possible.
Rhabdomyolysis/myoglobinuria may cause acute renal failure. 		Exercise test: ? No treatment information in references given. NLM/GHR:PGAM2
OMIM: PGAM2
NLM/GHR:GSD X
OMIM: GSD X
GARD: GSD X
ORPHA: GSD X
Glycolysis step 9
Enolase  1
(Alpha-enolase,
α-enolase) 		ENO1:
RBCs
Enolase deficiency
(α-enolase deficiency, alpha-enolase deficiency) 		Hemolytic anemia. OMIM: ENO1
Glycolysis step 9
Enolase  1
(Alpha-enolase,
α-enolase) 		ENO1
Unclear role in: 		Autoimmunity, unclear role. See respective conditions See respective conditions OMIM: ENO1
Glycolysis step 9
Enolase  3
(Beta-enolase,
β-enolase) 		ENO3:
Muscle
GSD type XIII
(GSD 13, β-enolase deficiency, beta-enolase deficiency, enolase 3 deficiency, muscle enolase deficiency) 		Myopathy. Exercise-induced myalgias, generalized muscle weakness and fatigability. Exercise test: No rise of lactate.
Biopsy: Focal sarcoplasmic accumulation of glycogen-beta particles. Immunohistochemistry and immunoblotting show reduced beta-enolase protein. 		No treatment information in references given. NLM/GHR:ENO3
OMIM: ENO3
OMIM: GSD XIII
GARD: GSD XIII
ORPHA: GSD XIII
Glycolysis step 10
Pyruvate kinase 		PKLR:
RBCs, liver
Pyruvate kinase deficiency
(PK deficiency, PKD) 		Hemolytic anemia. NLM/GHR:PKLR
OMIM: PKLR
NLM/GHR:PKD
OMIM: PKD
GARD: PKD
ORPHA: PKD

The pyruvate created by glycolysis (in the cytosol) is transported (together with a proton) to the mitochondrion for further energy extraction.

Under anaerobic conditions (without the use of oxygen) most if not all of the pyruvate is converted into lactate (furthermore producing NAD+ at the same time).

Under aerobic conditions (with the use of oxygen) only part of the pyruvate is converted to lactate; the pyruvate not converted feeds the citric acid cycle (CAC); both via pyruvate dehydrogenase (PDC, with Acetyl-CoA as intermediate) and via pyruvate decarboxylation - this will create further ATP and NADH for the cell's use.

The pentose phosphate pathway (HMP Shunt) is connected to the glycolysis pathway, and can convert substrates to and from the glycolysis pathway. It generates NADPH and pentoses (5-carbon sugars) as well as ribose 5-phosphate, a precursor for the synthesis of nucleotides. While the pentose phosphate pathway does involve oxidation of glucose, its primary role is anabolic rather than catabolic. The pathway is especially important in red blood cells (erythrocytes).

Transport proteins move substrates through cellular membranes. A glucose transporter (GLUT) protein is needed to assist glucose into (and in the liver and kidneys, also out of) the cell. De Vivo disease (GLUT1 deficiency) is a deficiency of GLUT1, which is needed to transport glucose across the blood-brain barrier. Fanconi-Bickel syndrome (GLUT2 deficiency, formally known as GSD-XI) is a deficiency of GLUT2, which is needed for the transport of glucose between liver and blood.

Mitochondrial pyruvate carrier deficiency (MPYCD) is a metabolic disorder, in which the transport of pyruvate from the cytosol to the mitochondria is affected (gene SLC54A1/BRP44L/MPC1 [5] ); the deficiency is characterized by delayed psychomotor development and lactic acidosis with a normal lactate/pyruvate ratio resulting from impaired mitochondrial pyruvate oxidation. [6] A similar disease is also seen in mutations of gene SLC54A2/BRP44/MPC2. [7]

The gene SLC16A1/MCT1 is responsible for transporting lactate across membranes. Mutations in the monocarboxylate transporter 1 (MCT1) gene have been associated with three diseases: hyperinsulinemic hypoglycemia, familial 7 (HHF7); monocarboxylate transporter 1 deficiency (MCTD1); and erythrocyte lactate transporter defect (formerly, myopathy due to lactate transport defect). [8]

(See also bioenergetic systems.)

Related enzymatic function

Enzyme
(Relation) 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Management and treatment References
and links
Pyruvate dehydrogenation / decarboxylation.
Pyruvate dehydrogenase complex 		PDHA1, DLD, PDHX, PDHB, DLAT, PDP1, LIAS
Systemic/various
Pyruvate dehydrogenase deficiency
(PDHA deficiency, PDHAD, ataxia with lactic acidosis, intermittent ataxia with pyruvate dehydrogenase deficiency, pyruvate dehydrogenase complex deficiency, pyruvate decarboxylase deficiency, pyruvate dehydrogenase lipoic acid synthetase deficiency (PDHLD), some forms of Leigh Syndrome (genes PDHA1 and DLD)) 		2 major presentations: metabolic and neurologic. Between these 2 major presentations, there is a continuous spectrum of intermediate forms. [9] Those with predominantly neurological symptoms fit within the category of Leigh Syndrome. [9]

Broad clinical spectrum: From fatal lactic acidosis in the newborn to chronic neurologic dysfunction with structural abnormalities in the central nervous system without systemic acidosis. Most common cause of primary lactic acidosis in children.

NLM/GHR:PDHA1
OMIM: PDHA1

OMIM: DLD OMIM: PDHX OMIM: PDHB OMIM: DLAT OMIM: PDP1

OMIM: LIAS
NLM/GHR:PDHAD
OMIM: Leigh Syndrome

OMIM: PDHAD OMIM: DLDD OMIM: PDHXD OMIM: PDHBD
OMIM: PDHDD

OMIM: PDHPD

OMIM: PDHLD

Inter-conversion of pyruvate and lactate.
Lactate dehydrogenase A 		LDHA:
Muscle
GSD type XI
(GSD 11, lactate dehydrogenase deficiency, LDH deficiency) 		Myopathy. Exercise intolerance.

Note: Deficiency of dehydrogenase-B (LDHB) has been observed as asymptomatic.

Exercise test: Increased pyruvate, but no rise of lactate. No treatment information in references given. NLM/GHR:LDHA
OMIM: LDHA
NLM/GHR: GSD 11
OMIM: GSD 11
ORPHA: GSD 11
Inter-conversion between the pentose phosphate pathway and the glycolysis pathway (Fructose-6-P, Glyceraldehyde-3-P, Erythrose-4-P, Xylulose-5-P, and Ribose-5-P)
Transketolase 		TKT: multi-organ
Transketolase Deficiency (SDDHD [Short Stature, Developmental Delay, and congenital Heart Defects])		Developmental delay and intellectual disability, delayed or absent speech, short stature, and congenital heart defects. Additional features reported.Elevated plasma and urinary polyols (erythritol, arabitol, and ribitol) and urinary sugar-phosphates (ribose-5-phosphate and xylulose/ribulose-5-phosphate). Biopsy shows absent or low TKT.OMIM: SDDHD

ORPHA: TKT

Gluconeogenesis

Gluconeogenesis step
Enzyme 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Treatment References
and links
Gluconeogenesis step 1: Conversion of pyruvate into oxaloacetate
Pyruvate carboxylase 		PC: Liver
Pyruvate carboxylase deficiency types A, B, & C

(Leigh necrotizing encephalopathy due to pyruvate carboxylase deficiency, Ataxia with lactic acidosis II)

Lactic acidosis, hyperammonemia, hypoglycemia, hepatomegaly, neurological problems, hypotonia, reduced ketone synthesis, and demyelination of neurons.Some may respond to thiamine treatmentOMIM: PC
OMIM: PC deficiency
Gluconeogenesis step 8
Fructose 1,6-bisphosphatase 		FBP1:
Liver
Fructose bisphosphatase deficiency
(FBP1, Baker-Winegrad disease) 		Fasting hypoglycemia with lactic acidosis. Episodes of hyperventilation, apnea, and ketosis. Symptoms exacerbated by fructose, sucrose, and glycerol consumption. NLM/GHR:FBP1
OMIM: FBP1
OMIM: FBP1D
GARD: FBP1D
ORPHA: FBP1D
Gluconeogenesis step 10 (final step):
Conversion of G-1-P into glucose
Glucose 6-phosphatase 		G6PC:
Liver
SLC37A4  (G6PT1):
Liver
GSD type I
(GSD 1, von Gierke's disease, hepatorenal glycogenosis, glucose-6-phosphate deficiency, glucose-6-phosphate transport defect) 		Hypoglycemia and hepatomegaly. Growth retardation, delayed puberty, lactic acidemia, hyperlipidemia, hyperuricemia. In adults hepatic adenomas likely. Exercise test: Normal lactate and ammonia rise. [10] NLM/GHR:G6PC
OMIM: G6PC
NLM/GHR:SLC37A4
OMIM: SLC37A4
NLM/GHR:GSD 1
ORPHA: GSD 1
OMIM: GSD 1a
GARD: GSD 1a
ORPHA: GSD 1a
OMIM: GSD 1b
GARD: GSD 1b
ORPHA: GSD 1b
OMIM: GSD 1c/1d
Gluconeogenesis step 10 (final step):
Conversion of G-1-P into glucose
Glucose 6-phosphatase 		G6PC3:
WBCs, heart, others
Severe congenital neutropenia type 4
(SCN4, congenital agranulocytosis, congenital neutropenia, Kostmann's disease, severe congenital neutropenia-pulmonary hypertension-superficial venous angiectasis)
Dursun syndrome
(DURSS, pulmonary arterial hypertension-leukopenia-atrial septal defect syndrome) 		SCN4: A disorder of hematopoiesis. Maturation arrest of granulopoiesis at the level of promyelocytes. Neutropenia. Osteopenia, may lead to osteoporosis. Prone to recurrent infections. In some heart and genital abnormalities, cancerous conditions of the blood, seizures, developmental delay.
Dursun syndrome: Pulmonary arterial hypertension, cardiac abnormalities (including secundum-type atrial septal defect), intermittent neutropenia, lymphopenia, monocytosis and anemia. 		NLM/GHR:G6PC3
OMIM: G6PC3
NLM/GHR:SCN4
OMIM: SCN4
ORPHA: SCN4
ORPHA: DURSS

Glycogen metabolism

Glycogenesis

Glycogenesis.png

Glycogenesis is the metabolic pathway in which glycogen is created. Glycogen, which consists of branched long chains made out of the simple sugar glucose, is an energy storage form for carbohydrates in many human cells; this is most important in liver, muscle and certain brain cells.

The monosaccharide glucose-6-phosphate (G-6-P) is typically the input substance for glycogenesis. G-6-P is most commonly created from glucose by the action of the enzymes glucokinase (see glycolysis step 1) or hexokinase.

Through the action of several enzymes glycogen is built up:

  • G-6-P is converted into glucose-1-phosphate (G-1-P) by the action of phosphoglucomutase (PGM), passing through the obligatory intermediate glucose-1,6-bisphosphate.
  • G-1-P is converted into UDP-glucose by the action of the enzyme UDP-glucose pyrophosphorylase (UGP).
  • The enzyme glycogenin (GYG) is needed to create initial short glycogen chains, which are lengthened and branched by the other enzymes of glycogenesis.
  • Once eight glucose have been added to the glycogen chain, then glycogen synthase (GYS) can bind to the growing glycogen chain and add UDP-glucose to lengthen the glucogen chain.
  • Branches are made by glycogen branching enzyme (GBE), which transfers the end of the chain onto an earlier part, forming branches; these grow further grow by addition of more units.

On an alternative metabolic pathway the simple sugar galactose (Gal, which is typically derived from lactose) is converted by the enzyme galactokinase (GALK) to galactose-1-phosphate (Gal-1-P), which in turn is converted by the enzyme galactose-1-phosphate uridylyltransferase (GALT) to glucose-1-phosphate (G-1-P), which can also serve as input for glycogenesis – this bypasses the first step of glycogenesis (the enzyme phosphoglucomutase PGM).

Errors in glycogenesis can have different consequences on a cellular level:

  • Too little glycogen is produced, e.g. in GSD 0
  • The glycogen is badly formed and inaccessible, typically accumulating in the affected cells (e.g. polyglucosan bodies).

Depending on the affected cells and the extent of the deficiency, a wide range of symptoms and severities are the result.

Glycogenesis  step

Enzyme 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Treatment References
and links
Glycogenesis step:
Inter-conversion of G-1-P and G-6-P
Phosphoglucomutase  1
(Also last step of glycogenolysis) 		PGM1:
Liver, muscle, other
CDG syndrome type It
(CDG1T, PGM1-CDG, phosphoglucomutase 1 deficiency, PGM1 deficiency)
formerly: GSD type XIV
(GSD 14) 		Wide range of manifestations and severity. Commonly cleft lip and bifid uvula, hepatopathy, intermittent hypoglycemia, short stature, and exercise intolerance. DNA Test: mutation on PGM1.

Walk test: Second Wind phenomenon in some, [11] but not all. [12] Observable with treadmill and heart rate monitor. Muscle biopsy: shows glycogen accumulation. Blood test: Abnormal serum transferrin.

Non-ischemic forearm test: exercise-induced hyperammonemia with normal lactic acid rise. [13]

NLM/GHR:PGM1
OMIM: PGM1
OMIM: CDG 1T
ORPHA: CDG 1T
Glycogenesis step:
UDP-glucose synthesis
UDP-glucose pyrophosphorylase 		UGP2
Barakat-Perenthaler syndrome, EPILEPTIC ENCEPHALOPATHY, EARLY INFANTILE, 83; EIEE83 		severe autosomal recessive neurodevelopmental disorder, presenting in early life with intractable seizures, absence of virtually all developmental milestones, visual impairment, progressive microcephaly and minor dysmorphic features [14] - - OMIM: UGP2
Glycogenesis step:
Glycogen primer synthesis
Glycogenin 		GYG1:
Muscle
GSD type XV
(GSD 15, glycogenin deficiency)
Polyglucosan body myopathy type 2
(PGBM2) 		GSD 15: Myopathy, cardiomyopathy. Rare. Muscle weakness.
PGBM2: Myopathy. Proximal muscle weakness of the lower limbs, gait disturbances. Upper limbs and/or distal muscle weakness in some. Onset-age highly variable, slowly progressive. 		Exercise test: ?
Skeletal muscle biopsy: deficit of glycogen, predominance of slow-twitch, oxidative muscle fibers and mitochondrial proliferation.
Endomyocardial biopsy: hypertrophic cardiomyocytes, enlarged nuclei and large centrally located vacuoles containing periodic acid Schiff (PAS)-positive material (but ultrastructurally different from glycogen). Glycogen depletion in the remainder of the cytoplasm. 		No treatment information in references given. NLM/GHR:GYG1
OMIM: GYG1
OMIM: GSD 15
ORPHA: GSD 15

OMIM: PGBM2
ORPHA: PGBM2

Glycogenesis step:
Glucogen chain lengthening
Glycogen synthase 		GYS1:
Muscle
GSD type 0b
(GSD 0b, glycogen synthetase deficiency) 		Myopathy, cardiomyopathy, exercise intolerance. Exercise test: ? NLM/GHR:GYS2
OMIM: GYS2
OMIM: GSD 0B
ORPHA: GSD 0B
Glycogenesis step:
Glucogen chain lengthening
Glycogen synthase 		GYS2:
Liver
GSD type 0a
(GSD 0a, glycogen synthetase deficiency) 		Infancy or in early childhood onset. Morning fatigue and fasting hypoglycemia, hyperketonemia. Without hepatomegaly, hyperalaninemia or hyperlactacidemia. After meals, major hyperglycemia associated with lactate and alanine increase and hyperlipidemia. NLM/GHR:GYS2
OMIM: GYS2
NLM/GHR:GSD 0
OMIM: GSD 0A
ORPHA: GSD 0A
Glycogenesis step:
Glucogen chain branching
Glycogen branching enzyme 		GBE1:
Liver, muscle
GSD type IV
(GSD 4, Andersen's disease, amylopectinosis, brancher deficiency, glycogen branching enzyme deficiency, familial cirrhosis with deposition of abnormal glycogen) 		Different forms have been described: Activity of branching enzyme in erythrocytes. High-protein diet. Liver transplant for progressive liver disease. Cardiomyopathy may require certain medications. NLM/GHR:GBE1
OMIM: GBE1
NLM/GHR:GSD 4
OMIM: GSD 4
GARD: GSD 4
ORPHA: GSD 4
Glycogenesis step:
Glucogen chain branching
Glycogen branching enzyme 		GBE1:
Nerve cells
Adult polyglucosan body disease
(APBD) 		Neuropathy, affecting the central and peripheral nervous systems. Cognitive impairment, pyramidal tetraparesis, peripheral neuropathy, and neurogenic bladder. Peripheral neuropathy and progressive muscle weakness and stiffness (spasticity). Cerebellar dysfunction and extrapyramidal signs in some. Late-onset, slowly progressive. NLM/GHR:GBE1
OMIM: GBE1
NLM/GHR:APBD
OMIM: APBD
GARD: APBD
ORPHA: APBD

Glycogenolysis

Glycogen.svg

To access the energy stored as glycogen, cells use the metabolic pathway glycogenolysis (glycogen breakdown); this produces the simple sugar glucose-6-phosphate (G-6-P), from which cells can extract energy or build other substances (e.g. riboses).

G-6-P (which is also produced from glucose) acts as an input substance for:

(See also bioenergetic systems.)

An alternative to glycolysis is the Pentose phosphate pathway (PPP): Depending on cellular conditions the PPP can produce NADPH (another energy transport form in the cell) or synthesize riboses (important for substances based on ribose like e.g. RNA) - the PPP is for example important in red blood cells.

If glycogenolysis is taking place in the liver, G-6-P can be converted to glucose by the enzyme glucose 6-phosphatase (G6Pase); the glucose produced in the liver is then released to the bloodstream for use in other organs. Muscle cells in contrast do not have the enzyme glucose 6-phosphatase, so they cannot share their glycogen stores with the rest of the body.

In addition to glycogen breakdown with the glycogen debranching enzyme and the glycogen phosphorylase enzyme, cells also use the enzyme acid alpha-glucosidase in lysosomes to degrade glycogen.

A deficiency of an involved enzyme results in:

  • Accumulation of glycogen in the cells
  • Lack of cellular energy negatively affects the involved organs

Myophosphorylase (muscle glycogen phosphorylase) comes in two forms: form 'a' is phosphorylated by phosphorylase kinase, form 'b' is not phosphorylated. Form 'a' is de-phosphorylated into form 'b' by the enzyme phosphoprotein phosphatase, which is activated by elevated insulin.

Both forms 'a' and 'b' of myophosphorylase have two conformational states: active (R or relaxed) and inactive (T or tense). When either form 'a' or 'b' are in the active state, then the enzyme converts glycogen into glucose-1-phosphate.

Myophosphorylase-b is allosterically activated by elevated AMP within the cell, and allosterically inactivated by elevated ATP and/or glucose-6-phosphate. Myophosphorylase-a is active, unless allosterically inactivated by elevated glucose within the cell. In this way, myophosphorylase-a is the more active of the two forms as it will continue to convert glycogen into glucose-1-phosphate even with high levels of glycogen-6-phosphate and ATP. (See Glycogen phosphorylase§Regulation).

Glycogenolysis  step

Enzyme 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Treatment References
and links
Glycogenolysis  step:
Release of G-1-P
Glycogen phosphorylase 		PYGL:
Liver
GSD type VI
(GSD 6, Hers disease, hepatic glycogen phosphorylase deficiency, liver phosphorylase deficiency syndrome) 		Hepatomegaly, failure to thrive, growth retardation. No other developmental delay, no muscle involvement. Hypoglycemia, lactic acidosis, hyperlipidemia and ketosis during prolonged fasting periods. Infancy or childhood onset, symptoms tend to improve with age. NLM/GHR:PYGL
OMIM: PYGL
NLM/GHR:GSD 6
OMIM: GSD 6
GARD: GSD 6
ORPHA: GSD 6
Glycogenolysis  step:
Release of G-1-P
Glycogen phosphorylase 		PYGM:
Muscle
GSD type V
(GSD 5, McArdle's disease, muscle phosphorylase deficiency, myophosphorylase deficiency, PYGM deficiency) 		Myopathy: Exercise intolerance, symptoms tend to improve with rest. "Second wind" phenomenon in most. Some have hypertrophic calf muscles. [15] Rhabdomyolysis and myoglobinuria possible. Some have muscle weakness. Of those with muscle weakness, in two-thirds it worsens, however in some the muscle weakness is stable.
Onset forms: infant, child, adult. Infant-form most severe (e.g. progressive respiratory failure), adult-onset can be very mild (e.g. mainly poor stamina). 		Exercise test: Severely impaired rise of lactate. Normal or enhanced ammonia. [10] [4] [16] Exercise-induced inappropriate rapid heart rate and myogenic hyperuricemia. [17] [18] "Second wind" observable with treadmill and heart rate monitor in a 12-minute walk test. [19] [20]

Muscle biopsy: Skeletal muscle shows abnormal glycogen accumulation. [17]

DNA test: Autosomal recessive mutation on PYGM gene. [17]

NLM/GHR:PYGM
OMIM: PYGM
NLM/GHR:GSD 5
OMIM: GSD 5
GARD: GSD 5
ORPHA: GSD 5
Glycogenolysis  step:
Release of G-1-P
Glycogen phosphorylase 		PYGM:
Muscle
Myophosphorylase-a activity impaired, myophosphorylase-b preserved		Adult-onset muscle weakness. No exercise intolerance (which differentiates it from McArdle disease, GSD-V)DNA test: Autosomal dominant mutation on PYGM gene.

Muscle biopsy: Accumulation of the intermediate filament desmin in the myofibers

PMID: 32386344
Glycogenolysis  step:
Debranching of PLD
Glycogen debranching enzyme (GDE) 		AGL:
Liver, muscles
GSD type III
(GSD 3, Forbes disease, Cori disease, limit dextrinosis, glycogen debrancher deficiency, GDE deficiency, AGL deficiency) 		Infant or child onset, often at puberty some symptoms improve.
Liver: Hepatomegaly, growth retardation, hyperlipidemia, hypoglycemia. Occasional seizures related to hypoglycemia. Adult cirrhosis in some.
Muscle: Myopathy, muscular hypotonia, muscle wasting (distal, some limb-girdle, some proximal instead), hypertrophic cardiomyopathy. Slowly progressive muscle weakness.
GSD IIIa / IIIc: Liver and muscle
GSD IIIb / IIId: Liver only 		Exercise test: Severely impaired lactate response (muscle involvement). Normal or enhanced ammonia. [10] NLM/GHR:AGL
OMIM: AGL
NLM/GHR:GSD 3
OMIM: GSD 3
GARD: GSD 3
ORPHA: GSD 3
Affected enzymatic function

Enzyme
(Relation to glycogenolysis) 		Gene:
Organ(s)
Disease
(Synonyms) 		Reported symptoms.
Forms (if applicable)
Note: Not all patients have all symptoms; severity and presentation can vary.		Diagnostic tests Treatment References
and links
Glycogenolysis final step:
Release of G-1-P
Phosphorylase kinase, alpha 1
(Activation of liver glycogen phosphorylase, c.f. GSD 6) 		PHKA2:
Liver (GSD 9a)
PHKB:
Liver, Muscle (GSD 9b)
PHKG2:
Liver (GSD 9c)

GSD type IX
(GSD 9, phosphorylase b kinase deficiency, PhK deficiency, liver glycogenosis)
Formerly GSD type VIII (GSD 8)

GSD 9a: Liver form. Hepatomegaly, growth retardation, elevation of glutamate-pyruvate transaminase and glutamate-oxaloacetate transaminase, hypercholesterolemia, hypertriglyceridemia, and fasting hyperketosis. Improves with age, most adult patients are asymptomatic.
GSD 9a1: PhK deficiency in erythrocytes.
GSD 9a2: Normal PhK activity in erythrocytes.
GSD 9b: Liver and muscle form. Additionally mild myopathy like GSD 9d. Rare.
GSD 9c: Similar to GSD 9a, but tends to be more severe. In some hepatic fibrosis or cirrhosis. 		Exercise test: Muscle involvement see GSD 9d. NLM/GHR:PHKA2
OMIM: PHKA2
NLM/GHR:PHKB
OMIM: PHKB
NLM/GHR:PHKG2
OMIM: PHKG2
NLM/GHR:GSD 9
ORPHA: GSD 9
OMIM: GSD 9a1/9a2
ORPHA: GSD 9a/9c
OMIM: GSD 9b
ORPHA: GSD 9b
OMIM: GSD 9c
Glycogenolysis final step:
Release of G-1-P
Phosphorylase kinase, alpha 1
(Activation of muscle glycogen phosphorylase, c.f. GSD 5) 		PHKA1:
Muscle
GSD type IXd
(GSD 9d, phosphorylase b kinase deficiency, PhK deficiency, muscle glycogenosis)
Formerly GSD type VIII (GSD 8)
Formerly GSD type Vb (GSD 5b) [21] 		Myopathy. Exercise-induced muscle weakness or stiffness. Relative mild compared to other metabolic myopathies. Typically adult-onset, some asymptomatic in late adulthood. No liver involvement. Exercise test: Both impaired and normal lactate observed; possible submaximal/maximal or aerobic/anaerobic discrepancy. Normal or exaggerated ammonia response. [22] NLM/GHR:PHKA1
OMIM: PHKA1
NLM/GHR:GSD 9
OMIM: GSD 9d
ORPHA: GSD 9d/9e
Degradation of glycogen to glucose in lysosomes
Acid alpha-glucosidase

Lysosome-associated membrane protein 2
(Alternative pathway to glycogenolysis)

GAA:
Myopathy

LAMP2:

Myopathy
GSD type II
(GSD 2a, Pompe's disease, acid maltase deficiency, deficiency of lysosomal alpha-glucosidase, cardiomegalia glycogenica)

Danon disease (GSD 2b, Danon disease, lysosomal glycogen storage disease without acid maltase deficiency)

Symptoms of both GSD types IIa and IIb are very similar due to a defect in lysosomes. However, in type IIb, some show abnormal glycogen accumulation, but not all.

Classic infantile form (Pompe disease): Cardiomyopathy and muscular hypotonia. In some respiratory involvement.
Juvenile and adult form: Myopathy of the skeletal muscles. Exercise intolerance. Some similarity to limb-girdle dystrophy. In some respiratory involvement.
Non-classic infantile form: Less severe.

DNA test: Mutation in either GAA or LAMP2 gene. Pompe disease is autosomal recessive. Danon disease is X-linked dominant.

Muscle biopsy: Abnormal glycogen accumulation in lysosomes.

NLM/GHR:GAA
OMIM: GAAOMIM: LAMP2
NLM/GHR:GSD 2
OMIM: GSD 2
GARD: GSD 2
ORPHA: GSD 2OMIM: Danon disease

Mutations in the PRKAG2 gene have been traced to fatal congenital nonlysosomal cardiac glycogenosis; PRKAG2 is a noncatalytic gamma subunit of AMP-activated protein kinase (AMPK), which affects the release of G-1-P by phosphorylase kinase during nonlysosomal glycogenolysis. [23]

See also

Related Research Articles

<span class="mw-page-title-main">Glycolysis</span> Series of interconnected biochemical reactions

Glycolysis is the metabolic pathway that converts glucose into pyruvate, and in most organisms, occurs in the liquid part of cells, the cytosol. The free energy released in this process is used to form the high-energy molecules adenosine triphosphate (ATP) and reduced nicotinamide adenine dinucleotide (NADH). Glycolysis is a sequence of ten reactions catalyzed by enzymes.

<span class="mw-page-title-main">Anabolism</span> Set of metabolic pathways that construct molecules from smaller units

Anabolism is the set of metabolic pathways that construct molecules from smaller units. These reactions require energy, known also as an endergonic process. Anabolism is the building-up aspect of metabolism, whereas catabolism is the breaking-down aspect. Anabolism is usually synonymous with biosynthesis.

Gluconeogenesis (GNG) is a metabolic pathway that results in the biosynthesis of glucose from certain non-carbohydrate carbon substrates. It is a ubiquitous process, present in plants, animals, fungi, bacteria, and other microorganisms. In vertebrates, gluconeogenesis occurs mainly in the liver and, to a lesser extent, in the cortex of the kidneys. It is one of two primary mechanisms – the other being degradation of glycogen (glycogenolysis) – used by humans and many other animals to maintain blood sugar levels, avoiding low levels (hypoglycemia). In ruminants, because dietary carbohydrates tend to be metabolized by rumen organisms, gluconeogenesis occurs regardless of fasting, low-carbohydrate diets, exercise, etc. In many other animals, the process occurs during periods of fasting, starvation, low-carbohydrate diets, or intense exercise.

<span class="mw-page-title-main">Glucagon</span> Peptide hormone

Glucagon is a peptide hormone, produced by alpha cells of the pancreas. It raises the concentration of glucose and fatty acids in the bloodstream and is considered to be the main catabolic hormone of the body. It is also used as a medication to treat a number of health conditions. Its effect is opposite to that of insulin, which lowers extracellular glucose. It is produced from proglucagon, encoded by the GCG gene.

<span class="mw-page-title-main">Fructose bisphosphatase deficiency</span> Medical condition

In fructose bisphosphatase deficiency, there is not enough fructose bisphosphatase for gluconeogenesis to occur correctly. Glycolysis will still work, as it does not use this enzyme.

Carbohydrate metabolism is the whole of the biochemical processes responsible for the metabolic formation, breakdown, and interconversion of carbohydrates in living organisms.

<span class="mw-page-title-main">Phosphofructokinase 1</span> Class of enzymes

Phosphofructokinase-1 (PFK-1) is one of the most important regulatory enzymes of glycolysis. It is an allosteric enzyme made of 4 subunits and controlled by many activators and inhibitors. PFK-1 catalyzes the important "committed" step of glycolysis, the conversion of fructose 6-phosphate and ATP to fructose 1,6-bisphosphate and ADP. Glycolysis is the foundation for respiration, both anaerobic and aerobic. Because phosphofructokinase (PFK) catalyzes the ATP-dependent phosphorylation to convert fructose-6-phosphate into fructose 1,6-bisphosphate and ADP, it is one of the key regulatory steps of glycolysis. PFK is able to regulate glycolysis through allosteric inhibition, and in this way, the cell can increase or decrease the rate of glycolysis in response to the cell's energy requirements. For example, a high ratio of ATP to ADP will inhibit PFK and glycolysis. The key difference between the regulation of PFK in eukaryotes and prokaryotes is that in eukaryotes PFK is activated by fructose 2,6-bisphosphate. The purpose of fructose 2,6-bisphosphate is to supersede ATP inhibition, thus allowing eukaryotes to have greater sensitivity to regulation by hormones like glucagon and insulin.

<span class="mw-page-title-main">Pyruvate kinase</span> Class of enzymes

Pyruvate kinase is the enzyme involved in the last step of glycolysis. It catalyzes the transfer of a phosphate group from phosphoenolpyruvate (PEP) to adenosine diphosphate (ADP), yielding one molecule of pyruvate and one molecule of ATP. Pyruvate kinase was inappropriately named before it was recognized that it did not directly catalyze phosphorylation of pyruvate, which does not occur under physiological conditions. Pyruvate kinase is present in four distinct, tissue-specific isozymes in animals, each consisting of particular kinetic properties necessary to accommodate the variations in metabolic requirements of diverse tissues.

<span class="mw-page-title-main">Galactosemia</span> Medical condition

Galactosemia is a rare genetic metabolic disorder that affects an individual's ability to metabolize the sugar galactose properly. Galactosemia follows an autosomal recessive mode of inheritance that confers a deficiency in an enzyme responsible for adequate galactose degradation.

<span class="mw-page-title-main">Phosphoglucomutase</span>

Phosphoglucomutase is an enzyme that transfers a phosphate group on an α-D-glucose monomer from the 1 to the 6 position in the forward direction or the 6 to the 1 position in the reverse direction.

<span class="mw-page-title-main">Glucose 6-phosphate</span> Chemical compound

Glucose 6-phosphate is a glucose sugar phosphorylated at the hydroxy group on carbon 6. This dianion is very common in cells as the majority of glucose entering a cell will become phosphorylated in this way.

<span class="mw-page-title-main">Cori cycle</span> Series of interconnected biochemical reactions

The Cori cycle, named after its discoverers, Carl Ferdinand Cori and Gerty Cori, is a metabolic pathway in which lactate, produced by anaerobic glycolysis in muscles, is transported to the liver and converted to glucose, which then returns to the muscles and is cyclically metabolized back to lactate.

<span class="mw-page-title-main">Glucose 1-phosphate</span> Chemical compound

Glucose 1-phosphate is a glucose molecule with a phosphate group on the 1'-carbon. It can exist in either the α- or β-anomeric form.

The glucose cycle occurs primarily in the liver and is the dynamic balance between glucose and glucose 6-phosphate. This is important for maintaining a constant concentration of glucose in the blood stream.

<span class="mw-page-title-main">UTP—glucose-1-phosphate uridylyltransferase</span> Class of enzymes

UTP—glucose-1-phosphate uridylyltransferase also known as glucose-1-phosphate uridylyltransferase is an enzyme involved in carbohydrate metabolism. It synthesizes UDP-glucose from glucose-1-phosphate and UTP; i.e.,

<span class="mw-page-title-main">Sucrose phosphorylase</span>

Sucrose phosphorylase is an important enzyme in the metabolism of sucrose and regulation of other metabolic intermediates. Sucrose phosphorylase is in the class of hexosyltransferases. More specifically it has been placed in the retaining glycoside hydrolases family although it catalyzes a transglycosidation rather than hydrolysis. Sucrose phosphorylase catalyzes the conversion of sucrose to D-fructose and α-D-glucose-1-phosphate. It has been shown in multiple experiments that the enzyme catalyzes this conversion by a double displacement mechanism.

Glucose-1,6-bisphosphate synthase is a type of enzyme called a phosphotransferase and is involved in mammalian starch and sucrose metabolism. It catalyzes the transfer of a phosphate group from 1,3-bisphosphoglycerate to glucose-1-phosphate, yielding 3-phosphoglycerate and glucose-1,6-bisphosphate.

<span class="mw-page-title-main">Galactose epimerase deficiency</span> Medical condition

Galactose epimerase deficiency, also known as GALE deficiency, Galactosemia III and UDP-galactose-4-epimerase deficiency, is a rare, autosomal recessive form of galactosemia associated with a deficiency of the enzyme galactose epimerase.

Fructolysis refers to the metabolism of fructose from dietary sources. Though the metabolism of glucose through glycolysis uses many of the same enzymes and intermediate structures as those in fructolysis, the two sugars have very different metabolic fates in human metabolism. Unlike glucose, which is directly metabolized widely in the body, fructose is almost entirely metabolized in the liver in humans, where it is directed toward replenishment of liver glycogen and triglyceride synthesis. Under one percent of ingested fructose is directly converted to plasma triglyceride. 29% - 54% of fructose is converted in liver to glucose, and about a quarter of fructose is converted to lactate. 15% - 18% is converted to glycogen. Glucose and lactate are then used normally as energy to fuel cells all over the body.

Glyceroneogenesis is a metabolic pathway which synthesizes glycerol 3-phosphate or triglyceride from precursors other than glucose. Usually glycerol 3-phosphate is generated from glucose by glycolysis. Still, when glucose concentration drops in the cytosol, it is generated by another pathway called glyceroneogenesis. Glyceroneogenesis uses pyruvate, alanine, glutamine or any substances from the TCA cycle as precursors for glycerol 3-phosphate. Phosphoenolpyruvate carboxykinase (PEPC-K), which is an enzyme that catalyzes the decarboxylation of oxaloacetate to phosphoenolpyruvate is the main regulator for this pathway. Glyceroneogenesis can be observed in adipose tissue and also in the liver. A significant biochemical pathway regulates cytosolic lipid levels. Intense suppression of glyceroneogenesis may lead to metabolic disorders such as type 2 diabetes.

References

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  5. OMIM: BRP44L
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  21. GeneReviews: Phosphorylase Kinase Deficiency
  22. OMIM: GSD 9d
  23. OMIM: PRKAG2
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