Ming and dairy production are important activities in this region that were negatively impacted by the bovine vaccinia outbreaks. Our analyses showed that the C23L sequences of several Brazilian VACV isolates in the GKT137831 custom synthesis non-virulent group share a unique ten-nucleotide deletion. This deletion may cause a frameshift mutation, which would result in a stop-codon that may lead to a truncated C23L protein; although new studies are required focusing the C23L promoter and alternative transcription frames, this deletion can be considered to be a putative genetic marker for non-virulent Brazilian VACV isolates and may be used for the detection and molecular characterization of new isolates.AcknowledgmentsWe thank colleagues from the Laboratory of Virus for their excellent technical support. We thank Pro-Reitoria de Pesquisa da Universidade Federal de Minas Gerais (PRPq-UFMG) and Fundacao de Amparo a ` Pesquisa de Minas Gerais (FAPEMIG) for the financial support.Author ContributionsConceived and designed the experiments: BPD FGF GST EGK JSA. Performed the experiments: FLA GMFA DBO RKC MIMG APMFL BPD. Analyzed the data: FLA GMFA DBO JSA. Contributed reagents/ materials/analysis tools: FGF EGK. Wrote the paper: FLA GMFA FGF MIMG BPD EGK JSA.
G protein-coupled receptors (GPCRs) constitute the largest superfamily of cell surface receptors and regulate the cellular responses to a broad spectrum of extracellular signals, such as hormones, neurotransmitters, chemokines, proteinases, odorants, light and calcium ions [1?]. All GPCRs share a common molecular topology with a hydrophobic core of seven membranespanning a-helices, three intracellular loops, three extracellular loops, an N-terminus outside the cell, and a C-terminus inside the cell. The proper function of GPCRs is largely determined by the highly regulated intracellular trafficking of the receptors. GPCRs are synthesized in the ER and after proper folding and correct assembly, they transport to the cell surface en route through the Golgi apparatus and trans-Golgi network. As the first step in post-translational biogenesis, the efficiency of ER export of nascent GPCRs plays a crucial role in the regulation of maturation, cell-surface expression, and physiological functions of the receptors [5?]. Great progress has been made on the understanding of GPCR export from the ER over the past decade [5,7]. However, the underlying molecular mechanisms remain 10457188 much less-well Filgotinib web understood as compared with extensive studies on the events involved in the endocytic and recycling pathways [9?4]. It has been demonstrated that, similar 24195657 to many other plasma membrane proteins, GPCRs must first attain native conformation in order toexit from the ER. Incompletely or misfolded receptors are excluded from ER-derived transport vesicles by the ER quality control mechanism [15?7]. It is also clear that GPCR export from the ER is modulated by direct interactions with a multitude of regulatory proteins such as ER chaperones and receptor activity modifying proteins (RAMPs), which may stabilize receptor conformation, facilitate receptor maturation and promote receptor delivery to the plasma membrane [18?3]. More interestingly, a number of highly conserved, specific sequences or motifs embedded within the receptors have recently been indentified to dictate receptor export from the ER [24?3]. Although the molecular mechanisms underlying the function of these motifs remain elusive, they may modulate proper receptor folding in the ER o.Ming and dairy production are important activities in this region that were negatively impacted by the bovine vaccinia outbreaks. Our analyses showed that the C23L sequences of several Brazilian VACV isolates in the non-virulent group share a unique ten-nucleotide deletion. This deletion may cause a frameshift mutation, which would result in a stop-codon that may lead to a truncated C23L protein; although new studies are required focusing the C23L promoter and alternative transcription frames, this deletion can be considered to be a putative genetic marker for non-virulent Brazilian VACV isolates and may be used for the detection and molecular characterization of new isolates.AcknowledgmentsWe thank colleagues from the Laboratory of Virus for their excellent technical support. We thank Pro-Reitoria de Pesquisa da Universidade Federal de Minas Gerais (PRPq-UFMG) and Fundacao de Amparo a ` Pesquisa de Minas Gerais (FAPEMIG) for the financial support.Author ContributionsConceived and designed the experiments: BPD FGF GST EGK JSA. Performed the experiments: FLA GMFA DBO RKC MIMG APMFL BPD. Analyzed the data: FLA GMFA DBO JSA. Contributed reagents/ materials/analysis tools: FGF EGK. Wrote the paper: FLA GMFA FGF MIMG BPD EGK JSA.
G protein-coupled receptors (GPCRs) constitute the largest superfamily of cell surface receptors and regulate the cellular responses to a broad spectrum of extracellular signals, such as hormones, neurotransmitters, chemokines, proteinases, odorants, light and calcium ions [1?]. All GPCRs share a common molecular topology with a hydrophobic core of seven membranespanning a-helices, three intracellular loops, three extracellular loops, an N-terminus outside the cell, and a C-terminus inside the cell. The proper function of GPCRs is largely determined by the highly regulated intracellular trafficking of the receptors. GPCRs are synthesized in the ER and after proper folding and correct assembly, they transport to the cell surface en route through the Golgi apparatus and trans-Golgi network. As the first step in post-translational biogenesis, the efficiency of ER export of nascent GPCRs plays a crucial role in the regulation of maturation, cell-surface expression, and physiological functions of the receptors [5?]. Great progress has been made on the understanding of GPCR export from the ER over the past decade [5,7]. However, the underlying molecular mechanisms remain 10457188 much less-well understood as compared with extensive studies on the events involved in the endocytic and recycling pathways [9?4]. It has been demonstrated that, similar 24195657 to many other plasma membrane proteins, GPCRs must first attain native conformation in order toexit from the ER. Incompletely or misfolded receptors are excluded from ER-derived transport vesicles by the ER quality control mechanism [15?7]. It is also clear that GPCR export from the ER is modulated by direct interactions with a multitude of regulatory proteins such as ER chaperones and receptor activity modifying proteins (RAMPs), which may stabilize receptor conformation, facilitate receptor maturation and promote receptor delivery to the plasma membrane [18?3]. More interestingly, a number of highly conserved, specific sequences or motifs embedded within the receptors have recently been indentified to dictate receptor export from the ER [24?3]. Although the molecular mechanisms underlying the function of these motifs remain elusive, they may modulate proper receptor folding in the ER o.