Complete amino acid sequence of the neurone‐specific γ isozyme of enolase (NSE) from human brain and comparison with the non‐neuronal α form (NNE)

McALEESE, Sybil M.; Dunbar, Bryan; Fothergill, John E.; Hinks, Lesley J.; Day, Ian N.M.

doi:10.1111/j.1432-1033.1988.tb14465.x

Cited by 50 publications

(35 citation statements)

References 21 publications

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“…NSE is a cytosolic protein that functions as brain-specific glycolytic enzyme, and plays an important role in intracellular energy metabolism [48]. It is expressed by mature neurons and cells of neuronal origin, and thus regarded as a marker of the neuronal state [49,50], but becomes markedly expressed after brain injury [51]. It is reported that RV cause neuronal injury [20,22], and this may be a reason for the marked expression of the enolase, which may be deleterious to the normal function of the cerebellar cortical cells.…”

Section: Discussionmentioning

confidence: 99%

Rauwolfia vomitoria and Gongronema latifolium extracts influences cerebellar cortex

Ekong¹,

Nwakanma²

2017

Alzheimers Dement Cogn Neurol

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Oxidative stress and free radical production is an etiology to some neurodegenerative diseases which may be preventable by prior neuronal protection using herbs. Rauwolfia vomitoria and Gongronema latifolium are medicinal herbs with antioxidant, anti-diabetic and analgesic properties among others. While R. vomitoria acts as a brain stimulant, as well as a depressant, neurotoxic effects have also been reported, which G. latifolium has shown the potential to mitigate. This study therefore investigated the effects of the combination of R. vomitoria and G. latifolium on young rats' cerebellar cortex. Twenty young male Wistar rats (100-150 g) were divided equally into 4 groups (n=5). Oral doses of the vehicle (Tween 20™), ethanolic extracts of 200 mg/kg of R. vomitoria (RV), 200 mg/kg of G. latifolium (GL), and the combination of both (RV + GL) were given to the animals for 14 days. On day 15, the animals were sacrificed after ketamine sedation and perfusion-fixed with 10% buffered-formalin. The cerebella were excised and processed for histomorphology by silver impregnation technique and immunolabelled with anti-neuron specific enolase (NSE) and glial fibrillary acidic protein (GFAP). The histology results showed atrophied Purkinje and other neurons with increased NSE and GFAP expressions in the RV group, which were not as such in the GL and RV+GL groups, an indication of cerebellar cortical injury. In conclusion, RV was injurious to the cerebellar cortical neurons and also stimulated NSE and GFAP, but these RV-induced traumas were slightly mitigated with GL combination. This preliminary report of RV+GL combination may be considered an alternative to RV single treatment for better disease management and brain protection.

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Section: Discussionmentioning

confidence: 99%

Rauwolfia vomitoria and Gongronema latifolium extracts influences cerebellar cortex

Ekong¹,

Nwakanma²

2017

Alzheimers Dement Cogn Neurol

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“…Although there was a higher prevalence of positive proliferative responses against NSE in MS patients compared to that in controls, we did not find any difference in proliferative responses against NNE. Enolase is a glycolytic enzyme (2-phospho-D-glycerate hydrolase), which exists in three isoforms: α-enolase or NNE, which is ubiquitous, β-enolase, which is predominant in muscle, and γ-enolase of NSE, which is found in neurons, paraneuronal cells, and neuroendocrine cells (38,39). Recently, the important contribution of neurodegeneration to the pathogenesis of MS has been appreciated (40,41).…”

Section: Discussionmentioning

confidence: 99%

Enolase and Arrestin are Novel Nonmyelin Autoantigens in Multiple Sclerosis

et al. 2007

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Introduction-Although myelin autoimmunity is known to be a major factor in the pathogenesis of multiple sclerosis (MS), the role of nonmyelin antigens is less clear. Given the complexity of this disease, it is possible that autoimmunity against nonmyelin antigens also has a pathogenic role. Autoantibodies against enolase and arrestin have previously been reported in MS patients. The Tcell response to these antigens, however, has not been established.

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“…la and lb). Additionally, at these stringencies cDNA probes representing the N-or C-terminus of NSE [9] identified XbaI fragments of 5 kb and 0.8 kb respectively on Southern blots of AHGME (results not shown). The map of AHGME is shown in Fig.…”

Section: Resultsmentioning

confidence: 90%

“…Fragments derived from human NSE cDNA [9] and human NNE cDNA [8,10] were labelled by random priming for use as probes, as were genomic fragments derived from the clone AHGME described here. The latter probes were pre-reannealed with excess total human DNA prior to use [31].…”

Section: Reagentsmentioning

confidence: 99%

“…Three major tissue-specific isoforms of enolase have been identified in mammals and birds, y or neuron-specific enolase (NSE), expressed primarily in neurons, /J or musclespecific enolase (MSE), expressed in striated muscle, and a or non-neuronal enolase (NNE), expressed in foetal cells and other adult cell types. Detailed structural information concerning rat and human NSE and NNE has emerged from cDNA cloning [5][6][7][8][9][10][11], reaffirming the existence of three separate genes, of which only the rat NSE gene has been characterized so far [12]. The human gene loci have been named ENO] (NNE), EN02 (NSE) and EN03 (MSE), and chromosome in situ hybridization data are also suggestive of at least three loci [13].…”

Section: Introductionmentioning

confidence: 98%

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Molecular structure of the human muscle-specific enolase gene (ENO3)

Peshavaria

Day

1991

Biochemical Journal

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The single human gene for muscle-specific enolase was isolated and its structure was characterized, from which the mature mRNA transcript and encoded protein were also deduced. The gene contains 12 exons, spans approx. 6 kb and encodes a protein of 433 residues. The gene structure is similar to that found for the rat neuron-specific enolase gene, and the deduced protein aligns precisely with other enolase sequences, including the sequence of the only published crystallized enolase, yeast eno-1. The 5' boundary of the gene includes a 5' non-coding exon and is characterized by an upstream TATA-like box and CpG-rich region. This region contains potential recognition motifs for general transcriptional regulation involving Spl, activator protein 1 and 2, CCAAT box transcription factor/nuclear factor I and cyclic AMP, and for muscle-specific transcriptional regulation involving a CC(A + T-rich)6GG box, M-CAT-box CAATCCT and two myocyte-specific enhancer-binding factor 1 boxes.

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Complete amino acid sequence of the neurone‐specific γ isozyme of enolase (NSE) from human brain and comparison with the non‐neuronal α form (NNE)

Cited by 50 publications

References 21 publications

Rauwolfia vomitoria and Gongronema latifolium extracts influences cerebellar cortex

Rauwolfia vomitoria and Gongronema latifolium extracts influences cerebellar cortex

Enolase and Arrestin are Novel Nonmyelin Autoantigens in Multiple Sclerosis

Molecular structure of the human muscle-specific enolase gene (ENO3)

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