High-throughput construction method for expression vector of peptides for NMR study suited for isotopic labeling

Fusion protein constructs for labeled peptides were generated with the 114 amino acid thioredoxin (TRX), coupled with the incorporation of a histidine tag for affinity purification. Two tandem AhdI sites were designed in the multiple cloning site of the fusion vector according to our novel unidirectional TA cloning methodology named PRESAT-vector, allowing one-step background-free cloning of DNA fragments. Constructs were designed to incorporate the four residue sequence Ile-Asp-Gly-Arg to generate pure peptides following Factor Xa cleavage of the fusion protein. The system is efficient and cost-effective for isotopic labeling of peptides for heteronuclear NMR studies. Seven peptides of varying length, including pituitary adenylate cyclase activating polypeptide (PACAP), vasoactive intestinal peptide (VIP) and ubiquitin interacting motif (UIM), were expressed using this TRX fusion system to give soluble fusion protein constructs in all cases. Three alternative methods for the preparation of DNA fragments were applied depending on the length of the peptides, such as polymerase chain reaction, chemical synthesis or a 'semi-synthetic method', which is a combination of chemical synthesis and enzymatic extension. The ability easily to construct, express and purify recombinant peptides in a high-throughput manner will be of enormous benefit in areas of biomedical research and drug discovery.     

Redesigning a sweet protein: increased stability and renaturability

Monellin is one of two natural proteins from African berrieswith potent sweet taste. Monellin is the smaller of the two,and consists of two peptides. The protein loses sweetness whenheated above 50°C under acidic pH. Based on the crystalstructure of monellin we have fused the two chains into a singlechain using several different linkers copied and ‘transplanted’from the same molecule. One of the newly designed proteins isas potently sweet as the natural one, is more stable upon temperatureor pH changes, and renatures easily even after heating to 100°Cat low pH.     

A new approach to artificial and modified proteins: theory-based design, synthesis in a cell-free system and fast testing of structural properties by radiolabels

A novel approach to the creation of artificial and modifiedproteins has been elaborated. The approach includes a sequencedesign based on the molecular theory of protein secondary structureand folding patterns, gene expression in a cell-free systemand testing of structural properties of the synthesized polypeptidesat a nanogram level using radiolabelled chains. The approachhas been applied to a new synthetic protein albebetin whichhas been designed to form a 3-D fold which does not contradictany structural rule but has been never observed up to now innatural proteins. Using size-exclusion chromatography, urea-gradientelectrophoresis and limited proteolysis of a radiolabelled chain,it has been shown that the artificial protein is nearly as compactas natural proteins, cooperatively unfolds at high urea concentrationsand has some structural features of a definite structure consistentwith the designed one. As albebetin has been designed as consistingof two structural repeats, a ‘halfalbebetin’ (oneof these repeats) has also been synthesized and studied. Itwas shown that ‘half-albebetin’ is also compact     

Improved growth response of antibody/receptor chimera attained by the engineering of transmembrane domain

Structure-based design of antibody/cytokine receptor chimeras has permitted a growth signal transduction in response to non-natural ligands such as fluorescein-conjugated BSA as mimicry of cytokine-cytokine receptor systems. However, while tight on/off regulation is observed in the natural cytokine receptor systems, many chimeras constructed to date showed residual growth-promoting activity in the absence of ligands. Here we tried to reduce the basal growth signal intensity from a chimera by engineering the transmembrane domain (TM) that is thought to be involved in the interchain interaction of natural cytokine receptors. When the retroviral vectors encoding the chimeras with either the wild-type erythropoietin receptor (EpoR) TM or the one bearing two mutations in the leucine zipper motif were transduced to non-strictly interleukin-6-dependent 7TD1 cells, a tight antigen-dependent on/off regulation was attained, also demonstrating the first antigen-mediated genetically modified cell amplification of non-strictly factor-dependent cells. The results clearly indicate that the TM mutation is an effective means to improve the growth response of the antibody/receptor chimera.     

Polarity as a criterion in protein design

Hypothetical proteins can be tested computationally by determiningwhether or not the designed sequence-structure pair has thecharacteristics of a typical globular protein. We have developedsuch a test by deriving quantities with approximately constantvalue for all globular proteins, based on empirical analysisof the exposed and buried surfaces of 128 structurally knownproteins. The characteristic quantities that best appear tosegregate badly designed or deliberately misfolded proteinsfrom their properly folded natural relatives are the polar fractionof side chains on the protein surface and, independently, inthe protein interior. Three of the seven hypothetical structurestested here can be rejected as having too many polar side-chaingroups in the interior or too few on the protein surface. Inaddition, a recently designed nutritional protein is identifiedas being very much unlike globular proteins. These database-derivedcharacteristic quantities are useful in screening designed proteinsprior to experiment and may be useful in screening experimentallydetermined (X-ray, NMR) protein structures for possible errors.     

An intein-based genetic selection allows the construction of a high-quality library of binary patterned de novo protein sequences

Combinatorial libraries of synthetic DNA are increasingly being used to identify and evolve proteins with novel folds and functions. An effective strategy for maximizing the diversity of these libraries relies on the assembly of large genes from smaller fragments of synthetic DNA. To optimize library assembly and screening, it is desirable to remove from the synthetic libraries any sequences that contain unintended frameshifts or stop codons. Although genetic selection systems can be used to accomplish this task, the tendency of individual segments to yield misfolded or aggregated products can decrease the effectiveness of these selections. Furthermore, individual protein domains may misfold when removed from their native context. We report the development and characterization of an in vivo system to preselect sequences that encode uninterrupted gene segments regardless of the foldedness of the encoded polypeptide. In this system, the inserted synthetic gene segment is separated from an intein/thymidylate synthase (TS) reporter domain by a polyasparagine linker, thereby permitting the TS reporter to fold and function independently of the folding and function of the segment-encoded polypeptide. TS-deficient Escherichia coli host cells survive on selective medium only if the insert is uninterrupted and in-frame, thereby allowing selection and amplification of desired sequences. We demonstrate that this system can be used as a highly effective preselection tool for the production of large, diverse and high-quality libraries of de novo protein sequences.     

Expression in Escherichia coli of a synthetic gene coding for horse heart myoglobin

A gene for expression of horse heart myoglobin in Escherichiacoli has been constructed in one step from long synthetic oligonucleotides.The synthetic gene contains an efficient translation initiationsignal and used codons that are commonly found in E.coli. Uniquerestriction sites are placed throughout the gene. It has beeninserted in a phagemid vector and is expressed from the lacpromoter in E.coli at high efficiency, the soluble heme proteinrepresenting 10% of soluble protein. Two versions of horse heartmyoglobin were produced with aspartic acid or asparagine atresidue 122. Comparison of chromatographic mobilities of thesetwo proteins with authentic horse heart myoglobin identifiedaspartic acid as the correct residue 122. The availability ofthis gene, which is designed to facilitate oligonucleotide mutagenesisor cassette mutagenesis, will allow systematic structure—functionanalysis of horse heart myoglobin.     

Binding specificities of the GYF domains from two Saccharomyces cerevisiae paralogs

We have used multivariate statistics and z-scales to represent peptide sequences in a PLS-QSAR model of previously studied binding affinities [Kofler,M., Motzny,K. and Freund,C. (2005b) Mol. Cell. Proteomics, 4, 1797-1811.] of two GYF domains to an array of immobilized synthetic peptides. As a result, we established structural determinants of the binding specificities of the two proteins. Our model was used to define new sets of yeast proteins potentially interacting with Syh1 (YPL105C) and Smy2 (YBR172C). These sets were subsequently examined for co-occurrence of Gene Ontology terms, leading to suggest a group of likely interacting proteins with a common function in mRNA catabolism. Finally, subcellular localization of a GFP-fused Syh1 and Smy2 reinforced the possibility that these proteins reside in cytoplasmic sites of mRNA degradation, thereby providing experimental confirmation to the predictions from the model.     

Engineering a de novo-designed coiled-coil heterodimerization domain for the rapid detection, purification and characterization of recombinantly expressed peptides and proteins

Using the techniques of genetic engineering and the principlesof protein de novo design, we have developed a unique affinitymatrix protein tag system as a rapid, convenient and sensitivemethod to detect, purify and characterize newly expressed recombinantpeptides or proteins from cell extracts. The method utilizestwo de novo-designed linear peptide sequences that can selectivelydimerize to form the stable protein motif, the two-stranded-helical coiled-coil. In this method, a recombinant bacterialexpression vector pRLDE has been engineered so that one of thedimerization strands (E-coil) is expressed as a C-terminal fusiontag on newly expressed peptides or proteins, while the other(K-coil) is either biotin-labeled for detection in a Westernblot-type format or immobilized on an insoluble silica supportfor selective dimerization affinity chromatography. Recombinantlyexpressed peptides from Escherichia coli containing the dimerizationtag have been produced, detected and purified using this method.The recombinant peptides were easily and clearly identifiedusing the biotin-labeled coil, while the single-step affinitypurification results indicated the purity of the affinity purifiedexpressed peptides to be >95%, as assessed by reversed-phasechromatography. The stability of the dimerization domain alsoallows for the purified peptide to be left attached to the matrix,thus creating a new peptide-bound column that can be used tostudy peptide–protein or peptide–ligand interactions.Therefore this system offers a new alternative to existing peptideor protein fusion tags and demonstrates the utility of a denovo-designed system.     

Protein design for non-aqueous solvents

Improving protein stability in unnatural and suboptimal environmentsis a promising application of protein engineering technology.Carefully designed amino acid alterations may lead to dramaticpositive effects on the stability of proteins under highly perturbingconditions, such as in non-aqueous solvents. Applications ofbiocatalysts and proteins with specific binding capabilitiesin the chemical industry have been severely limited by constraintsplaced on the solvent environment. With the advent of convenientmethods for altering the amino acid composition and even synthesizingentirely new protein molecules, it is worthwhile to considerengineering proteins for stability in non-aqueous solvents.In order to identify the features that a protein would needfor stability in organic media, we have been studying the structureand properties of the hydrophobic protein crambin. Crambin isunique in that it is soluble and stable in very high concentrationsof polar organic solvents. Crambin and its water-soluble homologsoffer a powerful demonstration of protein engineering for non-aqueoussolvents. This paper describes the structural features thatcontribute to crambin's special properties. Based on these observationsand consideration of how non-aqueous solvents affect the interactionsimportant in protein folding, a set of rules for designing non-aqueoussolvent-stable proteins is proposed.     

A novel search method for protein sequence-structure relations using property profiles

In protein engineering and design it is very important thatresidues can be inspected in their specific environment. A standardrelational database system cannot serve this purpose adequatelybecause it cannot handle relations between individual residues.With SCAN3D we introduce a new database system for integratedsequence and structure analysis of proteins. It uses the relationalparadigm wherever possible. Its main power, however, stems fromthe ability to retrieve stretches of consecutive residues withcertain properties by comparing a property profile with allstretches of residues in the database, exploiting the orderedcharacter of proteins. In doing so, it bypasses the large numberof join operations that would be required by relational databasesystems. An additional advantage of using property profile matchingis that searches can be carried out allowing a pre-set numberof mismatches. Also, as the database is read-only, SCAN3D doesnot need interactive data update mechanisms. Queries typicalof a molecular engineering environment are demonstrated withspecific examples: analysis of peptides that induce local structure,analysis of site-dependent rotamers and residue-residue contactanalysis     

Nuclear magnetic resonance chemical shift: comparison of estimated secondary structures in peptides by nuclear magnetic resonance and circular dichroism

Traditionally, CD has been used extensively for peptides insecondary structure analysis. In recent years, NMR chemicalshifts and nuclear Overhauser enhancements have been widelyused in conjunction with CD to assess the secondary structuresof peptides and proteins; however, there are many instanceswhere the estimation of secondary structure contents differssignificantly between the two methods. In order to elucidatethe perceived differences between the two methods, secondarystructure estimations by CD and ¹H NMR chemical shifts werecompared for over 50 peptides. The linear peptides investigatedwere largely unstructured, {small tilde}15–50 residuesin size, and lacked stable tertiary conformation. These peptideswere studied in different solvent systems including water, alcohol—water,micelles and urea. A strong correlation exists for secondarystructure assessment by CD and NMR chemical shifts; however,an interesting trend of higher estimation of helical contentsby NMR was observed for peptide fragments from globular proteinsstudied in water. This may be a result of associative propertiesof these peptides in water. Addition-ally, a new method of quantitatingsecondary structure contents based on ¹H NMR chemical shiftsis reported.     

Distinctive properties of signal sequences from bacterial lipoproteins

We have compared a number of attributes (hydrophobicity, aminoacid size, charge and secondary structure propensities) of signalsequences from bacterial lipoproteins with the same attributesof signal peptides from other prokaryotic proteins (non-lipoproteins).Lipoprotein leader sequences tend to be shorter, more hydrophobicand bulky, and they have stronger conformational preferences,the most conspicuous being a predicted ß-turn comprisingpositions 2 or 3 of the mature protein. Another distinctivefeature is a maximum in the local energy profile between positions–1 and +2. With one exception (ß-lactamase III),the lipoproteins do not have Pro in their signal peptides, andthey tend to have fewer Ser and Thr but more Gly than non-lipoproteins.Lipoproteins also lack a net negative charge in the N-terminalregions of the mature proteins. The signal peptides of the bacteriocinplasmid-coded lysis proteins appear to be unique in that theyhave all the ascribed features of lipoprotein signals; thesecharacteristics can be used to guide signal peptide mutagenesisexperiments and to construct new secretion vehicles.     

Negatively charged purification tags for selective anion-exchange recovery

A novel strategy for the highly selective purification of recombinant fusion proteins using negatively charged protein domains, which were constructed by protein design, is described. A triple alpha-helical domain of 58 amino acids was used as scaffold. Far-ultraviolet circular dichroism measurements showed that the designed domains had very low alpha-helicity in a low-conductivity environment in contrast to the scaffold. The secondary structure could be induced by adding salt, giving a structure comparable to the parental molecule. Further studies showed that the new domains were able to bind to an anion exchanger even at pH values down to 5 and 6. Gene fusions between one of the designed domains and different target proteins, such as green fluorescent protein (GFP), maltose binding protein (MBP) and firefly luciferase, were also constructed. These gene products could be efficiently purified from whole cell lysates at pH 6 using anion-exchange chromatography.     

Rapid detection of antigen binding by antibody fragments expressed in the periplasm of Escherichia coli

Bacterial expression systems can greatly facilitate proteinengineering of antibodies. We have developed a system for high-levelexpression of antibodies, antibody fragments, or hybrid antibodieswith novel effector functions in the periplasm of Escherichiacoli. From 5 ml of cells, a simple extraction yields sufficientmaterial for SDS-gel electro-phoresis, detection and characterizationof hapten binding. To demonstrate our system, heavy-chain variableregions and 1 light chains of a mouse anti-NP antibody weresynthesized as hybrid proteins with a bacterial signal peptide(Omp F). Each chain is secreted into the periplasm where processing(cleavage of the signal peptide), folding and heterodimer associationtake place. Periplasmic proteins are released by cold osmoticshock, and hapten-binding activity is easily detected withoutfurther manipulation. The ease of genetic engineering in thissystem will facilitate the production of immunoglobulin derivativesdesigned for specific applications, and expression of thesemolecules in a native state will allow the rapid screening ofcombinatorial libraries and the results of mutagenesis.     

Prediction of signal peptides in archaea

Computational prediction of signal peptides (SPs) and theircleavage sites is of great importance in computational biology;however, currently there is no available method capable of predictingreliably the SPs of archaea, due to the limited amount of experimentallyverified proteins with SPs. We performed an extensive literaturesearch in order to identify archaeal proteins having experimentallyverified SP and managed to find 69 such proteins, the largestnumber ever reported. A detailed analysis of these sequencesrevealed some unique features of the SPs of archaea, such asthe unique amino acid composition of the hydrophobic regionwith a higher than expected occurrence of isoleucine, and acleavage site resembling more the sequences of gram-positiveswith almost equal amounts of alanine and valine at the position-3before the cleavage site and a dominant alanine at position-1,followed in abundance by serine and glycine. Using these proteinsas a training set, we trained a hidden Markov model method thatpredicts the presence of the SPs and their cleavage sites andalso discriminates such proteins from cytoplasmic and transmembraneones. The method performs satisfactorily, yielding a 35-foldcross-validation procedure, a sensitivity of 100% and specificity98.41% with the Matthews’ correlation coefficient beingequal to 0.964. This particular method is currently the onlyavailable method for the prediction of secretory SPs in archaea,and performs consistently and significantly better comparedwith other available predictors that were trained on sequencesof eukaryotic or bacterial origin. Searching 48 completely sequencedarchaeal genomes we identified 9437 putative SPs. The method,PRED-SIGNAL, and the results are freely available for academicusers at http://bioinformatics.biol.uoa.gr/PRED-SIGNAL/ andwe anticipate that it will be a valuable tool for the computationalanalysis of archaeal genomes.     

Design and facile production of recombinant resilin-like polypeptides: gene construction and a rapid protein purification method

Resilin is an elastic protein found in specialized regions of the cuticle of insects, which displays unique resilience and fatigue lifetime properties. As is the case with many elastomeric proteins, including elastin, gliadin and spider silks, resilin contains distinct repetitive domains that appear to confer elastic properties to the protein. Recent work within our laboratory has demonstrated that cloning and expression of exon 1 of the Drosophila melanogaster CG15920 gene, encoding a putative resilin-like protein, results in a recombinant protein that can be photochemically crosslinked to form a highly resilient, elastic biomaterial (Rec1 resilin). The current study describes a recursive cloning strategy for generating synthetic genes encoding multiple copies of consensus polypeptides, based on the repetitive domains within resilin-like genes from D. melanogaster and Anopheles gambiae. A simple non-chromatographic purification method that can be applied to these synthetic proteins and Rec1 is also reported. These methods for the design and purification of resilin-like periodic polypeptides will facilitate the future investigation of structural and functional properties of resilin, and the development of novel highly resilient biomaterials.     

Biased random mutagenesis of peptides: determination of mutation frequency by computer simulation

Cassette mutagenesis is a method of protein engineering whichgenerates a wide diversity of genetic variants that can be subjectedto either selection or screening. As long as the target sequenceto be modified is kept short (corresponding to four to six aminoacids), complete combinatorial libraries can be produced. Amajor problem arises when longer peptides are to be engineeredfor desired functions. In such situations the production ofa limited collection of variants can be helpful; thus, biasedrandom mutagenesis and ‘doping schemes’ have beenreported previously. Here we describe a computer algorithm thatenables the determination of the degree of phosphoramidite contaminationof nucleotide precursor reservoirs. Through simulation of biologicaltranslation, the algorithm allows the prediction of the effectof contamination levels on the number of mutations to occurfor any given peptide sequence. In this study the cholinergicbinding site was used as a model sequence (22 amino acids).Considerations, based on the computer program, are discussedregarding the efficient design of phage-display combinatoriallibraries.     

Fidelity of seryl-tRNA synthetase to binding of natural amino acids from HierDock first principles computations

Seryl-tRNA synthetase (SerRS) charges serine to tRNA(Ser) following the formation of a seryl adenylate intermediate, but the extent to which other non-cognate amino acids compete with serine to bind to SerRS or for the formation of the activated seryl adenylate intermediate is not known. To examine the mechanism of discrimination against non-cognate amino acids, we calculated the relative binding energies of the 20 natural amino acids to SerRS. Starting with the crystal structure of SerRS from Thermus thermophilus with seryl adenylate bound, we used the HierDock and SCREAM (Side-Chain Rotamer Energy Analysis Method) computational methods to predict the binding conformation and binding energy of each of the 20 natural amino acids in the binding site in the best-binding mode and the activating mode. The ordering of the calculated binding energies in the activated mode agrees with kinetic measurements in yeast SerRS that threonine will compete with serine for formation of the activated intermediate while alanine and glycine will not compete significantly. In addition, we predict that asparagine will compete with serine for formation of the activated intermediate. Experiments to check the accuracy of this prediction would be useful in further validating the use of HierDock and SCREAM for designing novel amino acids to incorporate into proteins and for determining mutations in aminoacyl-tRNA synthetase design to facilitate the incorporation of amino acid analogs into proteins.     

Computer-aided gene design

A computer program, which runs on MS-DOS personal computers,is described that assists in the design of synthetic genes codingfor proteins. The goal of the program is the design of a genewhich (0 contains as many unique restriction sites as possibleand (ii) uses a specific codon usage. The gene designed accordingto the criteria above is (i) suitable for ‘modular mutagenesis’experiments and (ii) optimized for expression. The program 'reverse-translates'protein sequences into degenerated DNA sequences, generatesa map of potential restriction sites and locates sequence positionswhere unique restriction sites can be accommodated. The nucleicacid sequence is then ‘refined’ according to a specificcodon usage to remove any degeneration. Unique restriction sites,if potentially present, can be ‘forced’ into thedegenerated nucleic acid sequence by using 'priority codes'assigned to different restriction sequences.