Your search keyword '"signal sequence"' showing total 9 results

1. Tail-extension following the termination codon is critical for release of the nascent chain from membrane-bound ribosomes in a reticulocyte lysate cell-free system

Author

Takahara, Michiyo, Sakaue, Haruka, Onishi, Yukiko, Yamagishi, Marifu, Kida, Yuichiro, and Sakaguchi, Masao

Subjects

*GENETIC code, *RIBOSOMES, *RETICULOCYTES, *PEPTIDYLTRANSFERASE, *GENETIC translation, *CELL membranes, *MESSENGER RNA

Abstract

Abstract: Nascent chain release from membrane-bound ribosomes by the termination codon was investigated using a cell-free translation system from rabbit supplemented with rough microsomal membrane vesicles. Chain release was extremely slow when mRNA ended with only the termination codon. Tail extension after the termination codon enhanced the release of the nascent chain. Release reached plateau levels with tail extension of 10 bases. This requirement was observed with all termination codons: TAA, TGA and TAG. Rapid release was also achieved by puromycin even in the absence of the extension. Efficient translation termination cannot be achieved in the presence of only a termination codon on the mRNA. Tail extension might be required for correct positioning of the termination codon in the ribosome and/or efficient recognition by release factors. [Copyright &y& Elsevier]

Published

2013

2. Effects of signal sequence on phage-displayed disulfide-stabilized single chain antibody variable fragment (sc-dsFv) libraries

Author

Lee, Yu-Ching, Chen, Ing-Chien, Yu, Chung-Ming, Huang, Yi-Jen, Hsu, Hung-Ju, and Yang, An-Suei

Subjects

*IMMUNOGLOBULINS, *SULFIDES, *IMMUNOTECHNOLOGY, *PEPTIDASE, *GENE expression, *BACTERIOPHAGES

Abstract

Abstract: Phage-displayed single chain variable fragment (scFv) libraries are powerful tools in antibody engineering. Disulfide-stabilized scFv (sc-dsFv) with an interface disulfide bond is structure-wise more stable than the corresponding scFv. A set of recently discovered signal sequences replacing the wild type (pelB) signal peptidase cleavage site in the c-region has been shown to be effective in rescuing the expression of sc-dsFv libraries on the phage surface. However, the effects of the other regions of the signal sequence on the expression of the sc-dsFv libraries and on the formation of the interface disulfide bond in the phage-displayed sc-dsFv have not been clear. In this work, selected novel signal sequence variants in the h-region were shown to be equally effective in promoting sc-dsFv library expression on the phage surface; the expression level and complexity of the sc-dsFv libraries were comparable to the corresponding scFv libraries produced with the wild-type (pelB) signal sequence. The interface disulfide bond in the phage-displayed sc-dsFv was proven to form to a large extent in the library variant ensemble generated with signal sequence variants in both the h-region and the c-region. The sc-dsFv engineering platform established in this work can be applied to many of the known scFv molecules which are in need of a more stable version for the applications under harsh conditions or for longer shelf-life. [Copyright &y& Elsevier]

Published

2011

3. A synergistic effect of suppressive CGG codon in +2 position and downstream CAT repeats for efficient heterologous protein expression in Escherichia coli

Author

Pai, Vaishnavo Rabindranath and Murugan, Vadivel

Subjects

*ESCHERICHIA, *ESCHERICHIA coli, *ENTEROBACTERIACEAE, *GRAM-negative bacteria

Abstract

Abstract: The negative effect of NGG codons at +2 position has been well documented for the down regulation of recombinant protein expression in Escherichia coli. But this is not true when certain specific sequences are present in the downstream of NGG codons. This has been proved in our study while expressing human Erythropoietin (EPO) in E. coli GJ1158. Towards this, nine recombinant constructs were made and their expression profile was compared. In our results, we found that the suppressive nature of NGG codon (GGG, CGG) in the +2 position was overcome by imposing a downstream CAT repeat motif. The expression of EPO levels is higher in the constructs having the combination of both CGG codon at 2nd position and CAT repeats than the other constructs having either CGG or CAT repeat alone. In addition, it is also interesting to note that increasing number of CAT repeats shows increased expression levels. [Copyright &y& Elsevier]

Published

2008

4. Human ABC transporter isoform B6 (ABCB6) localizes primarily in the Golgi apparatus

Author

Tsuchida, Masashi, Emi, Yoshikazu, Kida, Yuichiro, and Sakaguchi, Masao

Subjects

*ATP-binding cassette transporters, *GOLGI apparatus, *MITOCHONDRIA, *HYDROPHOBIC surfaces

Abstract

Abstract: Human ATP-binding cassette transporter isoform B6 (ABCB6) has been proposed to be situated in both the inner and outer membranes of mitochondria. These inconsistent observations of submitochondrial localization have led to conflicting interpretation in view of directions of transport facilitated by ABCB6. We show here that ABCB6 has an N-terminal hydrophobic region of 220 residues that functions as a primary determinant of co-translational targeting to the endoplasmic reticulum (ER), but it does not have any known features of a mitochondrial targeting sequence. We defined the potential role of this hydrophobic extension of ABCB6 by glycosylation site mapping experiments, and demonstrated that the first hydrophobic segment acts as a type I signal-anchor sequence, which mediates N-terminal translocation through the ER membrane. Laser scanning microscopic observation revealed that ABCB6 did not co-localize with mitochondrial staining. Rather, it localized in the ER-derived and brefeldin A-sensitive perinuclear compartments, mainly in the Golgi apparatus. [Copyright &y& Elsevier]

Published

2008

5. Secretory signal sequence non-optimal codons are required for expression and export of β-lactamase

Author

Zalucki, Yaramah M., Gittins, Karlee L., and Jennings, Michael P.

Subjects

*GENE expression, *ESCHERICHIA coli, *BETA lactam antibiotics, *PROTEOLYTIC enzymes

Abstract

Abstract: In this study we altered the codon usage in the signal sequence of the bla gene, encoding β-lactamase in Escherichia coli. Changing all of the thirteen non-optimal codons to optimal lowered expression 4-fold as measured by minimum inhibitory concentration (MIC) to the β-lactam antibiotic ampicillin. The difference in ampicillin resistance was reduced at 28°C compared to expression at 37°C, suggesting that the optimised bla allele is misfolded and degraded by heat-shock regulated proteases. A screen was carried out, designed specifically to identify revertants with changes in codon usage resulting in higher MIC to ampicillin. The nine revertants revealed by this method all had optimal to non-optimal codon changes in the signal sequence. These results, and those of our previous study with maltose binding protein model system, confirm that non-optimal codons are important for expression and export of secretory proteins via both the SecB-dependent and -independent pathways. [Copyright &y& Elsevier]

Published

2008

6. Specific expression of GFPuv-β1,3-N-acetylglucosaminyltransferase 2 fusion protein in fat body of Bombyx mori silkworm larvae using signal peptide

Author

Kato, Tatsuya and Park, Enoch Y.

Subjects

*GENE expression, *GREEN fluorescent protein, *SIGNAL peptidases, *GENE fusion

Abstract

Abstract: Bombyxin (bx) and prophenoloxidase-activating enzyme (ppae) signal peptides from Bombyx mori, their modified signal peptides, and synthetic signal peptides were investigated for the secretion of GFPuv-β1,3-N-acetylglucosaminyltransferase 2 (GGT2) fusion protein in B. mori Bm5 cells and silkworm larvae using cysteine protease deficient B. mori multiple nucleopolyhedrovirus (BmMNPV-CP− ) and its bacmid. The secretion efficiencies of all signal peptides were 15–30% in Bm5 cells and 24–30% in silkworm larvae, while that of the +16 signal peptide was 0% in Bm5 cells and 1% in silkworm larvae. The fusion protein that contained the +16 signal peptide was expressed specifically in the endoplasmic reticulum (ER) and in the fractions of cell precipitations. Ninety-four percent of total intracellular β1,3-N-acetylglucosaminyltransferase (β3GnT) activity was detected in cell precipitations following the 600, 8000, and 114,000g centrifugations. In the case of the +38 signal peptide, 60% of total intracellular activity was detected in the supernatant from the 114,000g spin, and only 1% was found in the precipitate. Our results suggest that the +16 signal peptide might be situated in the transmembrane region and not cleaved by signal peptidase in silkworm or B. mori cells. Therefore, the fusion protein connected to the +16 signal peptide stayed in the fat body of silkworm larvae with biological function, and was not secreted extracellularly. [Copyright &y& Elsevier]

Published

2007

7. Experimental confirmation of a key role for non-optimal codons in protein export

Author

Zalucki, Yaramah M. and Jennings, Michael P.

Subjects

*CARRIER proteins, *TRANSFER RNA, *ESCHERICHIA coli, *PROTEOLYTIC enzymes

Abstract

Abstract: Non-optimal codons are defined by low usage and low abundance of corresponding tRNA, and have an established role in translational pausing to allow the correct folding of proteins. Our previous work reported a striking abundance of non-optimal codons in the signal sequences of secretory proteins exported via the sec-dependent pathway in Escherichia coli. In the current study the signal sequence of maltose-binding protein (MBP) was altered so that non-optimal codons were substituted with the most optimal codon from their synonymous codon family. The expression of MBP from the optimized allele (malE-opt) was significantly less than wild-type malE. Expression of MBP from malE-opt was partially restored in a range of cytoplasmic and periplasmic protease deficient strains, confirming that reduced expression of MBP in malE-opt was due to its preferential degradation by cytoplasmic and periplasmic proteases. These data confirm a novel role for non-optimal codon usage in secretion by slowing the rate of translation across the N-terminal signal sequence to facilitate proper folding of the secreted protein. [Copyright &y& Elsevier]

Published

2007

8. Influenza A H5N1 hemagglutinin cleavable signal sequence substitutions

Author

Weltman, Joel K., Skowron, Gail, and Loriot, George B.

Subjects

*INFLUENZA, *RESPIRATORY infections, *VIRUS diseases, *NUCLEOTIDES

Abstract

Abstract: Eleven influenza A H5N1 hemagglutinin N-terminal cleavable signal sequences, coded by single nucleotide substitutions relative to reference A/Viet Nam/1203/2004, were identified by BLASTN search of GenBank and were characterized by molecular modeling. The signal sequences statistically segregated into two classes of states. Members of one class were uncharged and conformationally compact while members of the second class each carried a 2+ electric charge and were conformationally extended. Virtual signal sequences, not found on GenBank and based upon hypothetical transversions in the third codon, had molecular characteristics intermediate to those of the two classes of actual signal sequences. The high incidence of non-synonymous substitutions (63.6%), the high transition/transversion ratio (10/1) and the results of molecular modeling all suggest that the N-terminal cleavable signal sequence is mutationally evolving more rapidly than proteins which must assume specific conformational states in the mature influenza virion. [Copyright &y& Elsevier]

Published

2007

9. Identification and characterization of two mature isoforms of retinoschisin in murine retina

Author

Vijayasarathy, Camasamudram, Gawinowicz, Mary Ann, Zeng, Yong, Takada, Yuichiro, Bush, Ronald A., and Sieving, Paul A.

Subjects

*RETINA, *PROTEOLYTIC enzymes, *AMINO acids, *GENETIC translation

Abstract

Abstract: Retinoschisin (RS) is a 24kDa secreted protein expressed in retina and is required for the structural and functional integrity of the retina. RS has been predicted to serve as an adhesive protein but the precise molecular mechanism by which it functions in retina is not yet known. During investigations on structural and functional aspects of RS in murine retina using proteomic tools, we identified two isoforms of RS that differed in mass by 200Da with no apparent change in charge. Mass spectra and amino acid sequence analysis of the tryptic peptides revealed that these isoforms differed by two amino acids at the N-terminus which suggested processing of RS signal sequence at two cleavage sites by signal peptidase as the basic mechanism underlying the occurrence of two mature RS isoforms in retina. Bioinformatic analysis identified two potential cleavage sites (between amino acids 21–22 and 23–24) in RS signal sequence. The flexibility of the signal peptidase to cleave at two sites is correlated to the amino acid composition of the RS signal sequence. This finding represents a rare example of a naturally occurring signal sequence cleavage at more than one site in vivo. [Copyright &y& Elsevier]

Published

2006