Detailed glycan analysis of serum glycoproteins of patients with congenital disorders of glycosylation indicates the specific defective glycan processing step and provides an insight into pathogenesis

The fundamental importance of correct protein glycosylation is abundantly clear in a group of diseases known as congenital disorders of glycosylation (CDGs). In these diseases, many biological functions are compromised, giving rise to a wide range of severe clinical conditions. By performing detailed analyses of the total serum glycoproteins as well as isolated transferrin and IgG, we have directly correlated aberrant glycosylation with a faulty glycosylation processing step. In one patient the complete absence of complex type sugars was consistent with ablation of GlcNAcTase II activity. In another CDG type II patient, the identification of specific hybrid sugars suggested that the defective processing step was cell type-specific and involved the mannosidase III pathway. In each case, complementary serum proteome analyses revealed significant changes in some 31 glycoproteins, including components of the complement system. This biochemical approach to charting diseases that involve alterations in glycan processing provides a rapid indicator of the nature, severity, and cell type specificity of the suboptimal glycan processing steps; allows links to genetic mutations; indicates the expression levels of proteins; and gives insight into the pathways affected in the disease process.     

Neurogenic differentiation of human adipose-derived stem cells: Relevance of different signaling molecules,transcription factors,and key marker genes

Since numerous diseases affect the central nervous system and it has limited self-repair capability, a great interest in using stem cells as an alternative cell source is generated. Previous reports have shown the differentiation of adipose-derived stem cells in neuron-like cells and it has also been proved that the expression pattern of patterning, proneural, and neural factors, such as Pax6, Mash1, Ngn2, NeuroD1, Tbr2 and Tbr1, regulates and defines adult neurogenesis. Regarding this, we hypothesize that a functional parallelism between adult neurogenesis and neuronal differentiation of human adipose-derived stem cells exists. In this study we differentiate human adipose-derived stem cells into neuron-like cells and analyze the expression pattern of different patterning, proneural, neural and neurotransmitter genes, before and after neuronal differentiation. The neuron-like cells expressed neuronal markers, patterning and proneural factors characteristics of intermediate stages of neuronal differentiation. Thus we demonstrated that it is possible to differentiate adipose-derived stem cells in vitro into immature neuron-like cells and that this process is regulated in a similar way to adult neurogenesis. This may contribute to elucidate molecular mechanisms involved in neuronal differentiation of adult human non-neural cells, in aid of the development of potential therapeutic tools for diseases of the nervous system.     

Differential expression of disialic acids in the cerebellum of senile mice

It is known that disialic acids (diSia) are present in the mammalian brain. However, the precise anatomical distribution and the chronology of its expression along life are not well studied yet. It is accepted that the transfer of diSia in the brain is mediated mainly by the enzyme ST8Sia III (α2,8-sialyltransferase III). We studied the expression of diSia glycoepitopes and of the ST8Sia III gene in different structures of the mouse brain at different postnatal stages by immunohistochemistry and real-time polymerase chain reaction, respectively. C57BL/6 mice of different stages were used. Samples of hippocampus, olfactory bulb, cortex and cerebellum were processed for studies of molecular biology and immunohistochemistry. Histological analysis revealed an important decrease in diSia labeling in the senile cerebellum compared with other structures and stages (P???0.001). In concordance with these results, a significant decrease in ST8Sia III gene expression was found in the cerebellum of senile animals (P?相似文献   

Comparison of two protocols for field immobilization of white-eared opossums (<Emphasis Type="Italic">Didelphis albiventris</Emphasis>)

The aim of this study was to investigate the efficacy of two protocols for field immobilization of white-eared opossums (Didelphis albiventris) and compare their effects on immobilization, cardiopulmonary variables, and recovery times. Twenty one opossums were randomly divided into two groups; G1 received ketamine (15 mg kg^?1)-dexmedetomidine (0.15 mg kg^?1) intramuscularly (IM) and G2 received the ketamine-dexmedetomidine combination and isoflurane once induction was achieved. Oxygen was delivered by face mask (1.5 L minute^?1). Thirty minutes after induction, isoflurane was discontinued (G2) and both groups were administered atipamezole (1.5 mg kg^?1) IM. Respiratory (?_R) and heart rate (HR), oxyhemoglobin saturation (SpO₂), and rectal temperature (T) were recorded every 5 min. Induction time, time to first movement (RT₁), and time to achieve standing (RT₂) were recorded. ANOVA and non-parametric tests were used. Level of immobilization was assessed by observation of movements and evaluation of muscle relaxation. The mean induction time was 4.71 min. RT₁ and RT₂ were significantly longer in G2. No significant differences were found in SpO₂ or ?R. HR did not vary significantly along time, but was higher in G2. Rectal temperature did not show differences between treatments, but decreased significantly with time in G2. Four of nine animals in G1 showed movements, while no animals in G2 did and muscle relaxation was determined to be better in this latter group. Both protocols were adequate for short-term field immobilization, with minimal alterations of HR and T and relatively short recovery times. Isoflurane provided better immobilization with statistically significant prolongation of recovery times.     

Differences in the hypoxic contraction of small isolated pulmonary arteries of cat and rabbit

Summary In small (<300 m diameter) pulmonary arterial (PA) rings isolated from the cat, hypoxia induced a transient contraction (250±120 mg, n=7), whereas in rings of rabbit PA of the same size, hypoxia had no significant effect (n=19). Precontraction by 40 mmol KCl · l^-1, noradrenaline (NA) 10^-6 mol · l^-1, or histamine (His 10^-5 mol · l^-1) did not modify this difference between the two species and did not potentiate the hypoxic contraction of small rings of the cat PA. Large rabbit pulmonary arterial segments (300–2000 m) exhibited no response to hypoxia before precontraction (n=15). In the presence of procaine (2%) rabbit PA rings (n=6, small) exhibited no hypoxic contraction. These results in vitro reflect previous in vivo observations.Abbreviations Ach acetylcholine - cGMP cyclic guanosine monophosphate - ED ₅₀ half maximal concentration - EGTA ethylene glycol-bis(2-amino-ethylether)-N,N,N,N-tetraacetic acid - HEPES N-hydroxyethylpiperazine-N-ethanesulfonic acid - His histamine - NA noradrenaline - PA pulmonary artery - PO ₂ partial pressure of oxygen - PRO procaine - STD standard deviation     

Squirrel monkey cytomegalovirus antibodies in free-ranging black howler monkeys (Alouatta caraya), Misiones, Argentina

Serum from four black howler monkeys (Alouatta caraya) was screened for antibodies to seven viruses by dot immunoassay. Cytomegalovirus antibodies were detected in three of four individuals and provide the first evidence of exposure by black howler monkeys to this virus.     

Prevalence of CYP2C9 and VKORC1 alleles in the Argentine population and implications for prescribing dosages of anticoagulants

Dicumarinic oral anticoagulants have a narrow therapeutic range and a great individual variability in response, which makes calculation of the correct dose difficult and critical. Genetic factors involved in this variability include polymorphisms of genes that encode the metabolic enzyme CYP2C9 and the target enzyme vitamin K epoxide reductase complex 1 (VKORC1); these polymorphisms can be associated with reduced enzymatic expression. We examined the frequency of the most relevant variants encoding CYP2C9 (alleles *1, *2 and *3) and VKORC1 (SNP -1639A>G) in the Argentinian population. Molecular typing was performed by PCR-RFLP on a randomly selected sample of 101 healthy volunteers from the Hospital Italiano de Buenos Aires gene bank. Fifty-seven subjects were identified as homozygous for CYP2C9*1 and 14 for *2, while 24 and 5 were heterozygous for *2 and *3 alleles; one individual was a composite heterozygote (*2/*3). When we examined VKORC1, 21 subjects were AA homozygous, 60 were AG heterozygotes and 20 were GG homozygotes. This is the first analysis of genotypic frequencies for CYP2C9 and VKORC1 performed in an Argentinian population. These allele prevalences are similar to what is known for Caucasian population, reflecting the European ancestor of our patient population, coming mostly from Buenos Aires city and surroundings. Knowledge of this prevalence information is instrumental for cost-effective pharmacogenomic testing in patients undergoing oral anticoagulation treatment.     

Effect of ryanodine on cardiac calcium current and calcium channel gating current.

The effects of 100 microM ryanodine on the L-type calcium channel were studied using the pacth-clamp technique in isolated guinea pig ventricular myocytes. The inactivation kinetics of the calcium current were slowed down in the presence of ryanodine in agreement with the blockade of the release of calcium from the sarcoplasmic reticulum by the drug. The I-V and steady-state inactivation curves of the calcium current were shifted to negative values by ryanodine. A similar shift was observed in the activation and inactivation curves of the intramembrane charge movement associated with the calcium channel. Due to this shift, ryanodine slightly reduced the maximal amount of displaced charge although it did not modify the transition from the inactivated to the activated state (i.e., charge movement repriming). This result is in notable contrast with that obtained in skeletal muscle, where it has been found that ryanodine interferes with charge movement repriming. These results provide additional evidence of the postulated differences between the architecture of the excitation-contraction coupling system in cardiac and skeletal muscle.