Vectors
Vectors
Vectors
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Plasmid biology:
Plasmids are widely used as cloning vehicles They are replicons and exist in double stranded state With both strands if DNA intact the molecules are
described as covalently closed circles or CCC DNA. However if one strand is intact the molecules are described as open circles or OC DNA. Not all plasmids exist as circular molecules, linear plasmids
have been found in a variety of organisms like Streptomyces and Borrelia burgdorferi.
To prevent the digestion by nucleases, the ends of linear 4/14/12
The interconversion of supercoiled, relaxed covalently closed circular DNA and open circular DNA.
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The ends of linear plasmids a protected by two general mechanisms: 1. There are repeated sequences ending in a terminal DNA hairloop (Borrelia) or 2. The ends are protected by covalent attachment of a protein (Streptomyces).
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Plasmids confer many phenotypic properties on their host cells. Plasmids without such phenotypic traits are called cryptic plasmids Plasmids with multiple copies inside a host cell are called relaxed plasmids, while those with fixed number of copies per cell are called stringent plasmids. Plasmids are also categorized as conjugative and nonconjugative plasmid- depending upon whether or not they carry a set of transfer genes, called the tra genes, which promote bacterial conjugation.
Generally conjugative plasmids have a high molecular weight 4/14/12 and are present as 1-3 copies per chromosome, where as non.
Plasmids encode only a few of the proteins required for their own replication and the other proteins are provided by the host cell.
The replication proteins encoded by the plasmid are located close to the ori.
Hence that is the only part necessary for the plasmid replication. The rest can be replaced by foreign sequences. Thus plasmids can be used as cloning vectors
Plasmids whose ori region is derived from plasmid Col E1 have restricted host range ie they can replicate in enteric bacteria such as E.coli or Salmonella.
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However some plasmids have a broad host range and these include RP4 and RSF1010.
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The plasmids of RP4 type replicate in most Gram-negative 4/14/12 bacteria, wherer they are readily transmitted by conjugation.
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Plasmids like RSF1010 are non conjugative but can be transformed into a wide range of Gram positive and Gran negative bacteria.
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Plasmids with a broad host range encode most of the proteins required for replication. They must be able to express these genes and thus their promoters and ribosome binding sites must have evolved such that they can be recognized in a diversity of bacterial families.
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Copy number of plasmid in a cell: The copy number of a plasmid is determined by regulating the initiation of plasmid replication.
Two mechanisms of control of initiation have been recognized: viz; regulation by antisense RNA and regulation by binding of essential proteins to repeated sequences called interons.
Most of the cloning vectors currently used carry an ori region derived from the Col E1 and copy-number control is mediated by antisense RNA.
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In such plasmids, the primer for DNA replication is a 555 base ribonucleotide molecule called RNA II, which forms the RNA-DNA hybrid at the ori.
RNA II can act as a primer only after it is cleaved by RNase H, which introduces the free 3 OH group.
Replication control is mediated by another small molecule called RNA I, which is encoded by the same region of DNA as RNA II, but by the complementary strand. Thus RNA II and RNA I are hence complementary to each other and can hybridize to form a double stranded RNA helix.
The formation of this double helix interferes with the processing of the RNA II by RNase H and hence replication does not begin.
Since RNA I is encoded by the plasmid, more of it is synthesized when the copy number is high. As the host cell grows and divides, the concentration of RNA I falls and the plasmid begins to replicate again.
In addition to RNA I, a plasmid-encoded protein Rop helps in maintaining the copy number. This protein forms a dimer, enhancing the pairing between RNA I and RNA II , so that the 4/14/12 processing of RNA II is inhibited even at relatively low
Regulation of replication of Col E1 derived plasmids. RNA II must be processed by RNase H before it can prime replication. Origin indicates the transition point between the RNA primer and DNA. Most of the time, RNA I binds to RNA II and inhibits the processing, thereby regulating the copy number. RNAI and RNAII are the promoters for RNA I and RNA II 4/14/12 transcription. The Rop protein dimer enhances the initial pairing of RNA I
In plasmid pSC101 and many of the broad-host range plasmids, the ori region contains 3-7 copies of an interon sequence which is 17-22 bp long.
Close to the ori region there is a gene called repA in pSC101, which encodes the RepA protein, which is the only plasmid encoded protein required for replication. It binds to the interons and initiates DNA synthesis.
First, the RepA protein represses its own synthesis by binding to its own promoter region and blocking transcription of its own gene.
If the copy-number is high, synthesis of RepA will be repressed. After cell division, the copy number and concentration of RepA will drop and replication will be initiated.
The ori region of pSC101. R1, R2 and R3 are the three interon sequences to which RepA binds to handcuff two plasmids. RepA autoregulates its own synthesis by binding to the inverted repeats IR1 and IR2. the location of the partitioning site par and the binding sites for the host protein DnaA are also shown. 4/14/12
Secondly, the RepA protein can link two plasmids together, by binding to their interon sequences, thereby preventing them from initiating replication.
By this mechanism the replication of interon plasmids will depend both on the concentration of RepA protein and the concentration of the plasmid themselves.
Stable maintenance of plasmids in cells: The loss of plasmids due to defective partitioning is called segregative instability. Naturally occurring plasmids are stably maintained because they contain a partitioning function, par, which ensures that they are stably maintained at each cell division. Such par regions are essential for stability of low-copy-number plasmids. The higher copy-number plasmid Col E1 also contain par region but this is deleted in many Col E1 derived cloning vectors 4/14/12 such as pBR322.
Though the copy number of vectors such as pBR322 is usually high, plasmid free cells arise under nutrient stress or other stress conditions. The par region from a plasmid can be cloned into pBR322, thereby stabilizing the plasmid.
DNA superhelicity is also involved in the partitioning mechanism. Plasmids lacking par locus (eg: pSC101 derivatives), exhibit a decreased super helical density as compared to the wild type.
Such plasmids are stabilized in E.coli by topA mutations, which increase negative DNA supercoiling. Conversely, DNA gyrase inhibitors and mutations in DNA gyrase increase the rate of loss of par-defective pSC101 derivatives.
Plasmid instability may also arise due to formation of multimeric forms of a plasmid. The mechanism that controls the copy number of a plasmid ensures a fixed number of plasmid origins per bacterium.
Cells containing multimeric plasmids have the same number of plasmid origins but fewer plasmid molecules, which leads to segregative instability if they lack a partitioning function. These multimeric forms are not seen with Col E1, which has a natural 4/14/12 of resolving multimers back to monomers. It contains a method
Plasmid incompatibility: It is the inability of two different plasmids to coexist in the same cell in the absence of selection pressure. Groups of plasmid which are mutually incompatible are considered to belong to the same incompatibility group (Inc). Plasmids are incompatible if they have same mechanism of replication control. By changing the sequence of the RNA I/ RNA II region of plasmids it is possible to change their incompatibility group. They will be incompatible if they share the same par region.
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Purification of Plasmid DNA: There are two methods for isolating pure plasmid DNA
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Isopycnic centrifugation of bacterial cleared lysates in a solution of Cesium chloride (Cscl) containing ethidium bromide. EtBr binds by intercalating between the DNA base pairs and causes the DNA to unwind. A CCC DNA has no free ends and so can limitedly unwind, thus limiting the amount of EtBr that binds. Linear DNA like the fragmented chromosomal DNA can bind to more EtBr molecules. The density of the DNA-EtBr complex decreases as more EtBr binds to the linear DNA. Hence, the CCC DNA has higher density at saturating concentrations of EtBr, than the linear DNA. Thus the plasmids can be separated from the linear chromosomal DNA.
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This method is by Birnboim and Doly. It makes use of the observation that there is a narrow range of pH (12.0-12.5) within which denaturation of linear DNA occurs. Plasmid containing cells are treated with lysozyme to weaken the cell wall and then lysed using SDS and NaOH. The chromosomal DNA denatures at this high alkaline pH. If the pH at this step is controlled properly, the plasmid DNA remains intact in the solution and chromosomal DNA gets precipitated out.
low molecular weight: easy to handle, present in high copy numbers and less chance of the vector having multiple restriction sites. .
pBR322 as a vector: It contains the ApR and TcR genes of the RSF2124 and pSC101 respectively, combined with replication elements of pMB1 and a Col E1 like plasmid.
The initially sequenced plasmid pBR322 was 4362 bp long. There are over 40 enzymes with unique cleavage sites on the pBR322 genome. The target sites of 11 enzymes lie within the tetracycline resistant gene and there are sites for a further two enzymes in the promoter of that gene. There are also sites for six enzymes within the ampicillin resistance gene. Thus cloning with these 19 enzymes results in inactivation of the ApR of TcR markers. E.coli cells transformed with plasmids with inserts in the TcR gene can be distinguished from those transformed with recircularized vector. The former are ApR and TcS, whereas latter are ApR and TcR. Replica plating can be performed to determine these.
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Cloning into the HindIII site of pBR322 result in loss of tetracycline resistance. However, in some recombinants, TcR is retained. This is because the HindIII site lies within the promoter rather than the coding sequence. Thus, if the cloned DNA carries a promoter like sequence, it is capable of initiating transcription of TcR gene. This technique had been used to search for promotercontaining fragments. Four structural domains can be recognized within E.coli promoters. These are: Position 1, from which RNA synthesis begins Position -6 to -12, the Pribnow box the region around basepair -35 the sequence between basepair -12 to -35. Although the HindIII site lies within the Pribnow box, the box is recreated on insertion of a foreign DNA. Thus when insertional inactivation occurs it must be the region from 4/14/12 -13 to -40.
Restriction map of pBR322 showing the location and direction of transcription of the ampicillin (Ap) and tetracycline (Tc) resistance loci, the ori and the Col E1 derived Rop gene. 4/14/12
Vectors derived from pBR322: Numerous different derivatives of pBR322 have been constructed to fulfill special cloning needs. pBR325: encodes chloramphenicol resistance in addition to ampicillin and tetracycline. It has a unique EcoRI site in the CmR gene. Further construction of improved vectors was simplified by the use of polylinkers or multiple cloning sites (MCS)pUC vectors. MCS is a short DNA sequence 2.8kb as in pUC19, carrying sites for many different RE. MCS increase the number of potential cloning sites by extending the range of RE that can be used. pUC vectors also incorporate the DNA sequence that permits rapid visual detection of an insert. The MCS is inserted into the lacZ sequence which encodes the promoter and the -peptide of the -galactosidase. The insertion of MCS into the lacZ fragment does not affect functioning of -peptide but cloning DNA fragments into the MSC does affect the functioning of -galactosidase. Therefore, 4/14/12 recombinants can be screened on medium containing X-gal.
Bacteriophage : It is the most studied virus of E.coli. The DNA of phage when isolated from the phage is a linear duplex molecule about 48.5 kbp. At each end are short stranded 5 projections of 12 nucleotides, which are complementary in sequence and by which the DNA adapts a circular structure when it is injected into the host cell. Thus DNA naturally has cohesive termini, which associate to form the cos site.
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Functionally related genes of phage are clustered together, except for the two regulatory genes N and Q. Genes on the left code for the head and tail proteins of the phage. Genes in the central region are concerned with recombination (red) and the process of lysogenization. Most of the central region is not required for replication or growth and hence can be replaced by genes of interest during cloning. To the right are genes concerned with regulation and prophage immunity to superinfection (N, cro, cI), followed by DNA synthesis (O,P), late 4/14/12 function regulation (Q) and host cell lysis (S,R).
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Control circuits of phage : Understanding of the control circuits of phage is important if the phage is to be used as a vector. It is possible to insert foreign DNA into the phage chromosome and in many a cases it is also expressed under the phage promoter. In lytic cycle, the transcription of the phage occurs in three stages: Early, middle and late. Early gene transcription establishes the lytic cycle, middle gene products replicate and recombine the DNA and late gene products pack the DNA into mature phage particles.
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Following infection transcription proceeds from major promoters PL and PR. This transcription is subject to repression by the product of the cI gene and in a lysogen this repression is the basis of immunity to superinfecting . The early infection transcripts stop at termination sites tL and tR1. The site tR2 stops any transcript that escapes tR1. Lambda switches from early to middle stage transcription by anti-termination. The N gene product expressed from PL directs this switch. It interacts with RNA polymerase and antagonizing the action of host termination protein , permits it to ignore the stop signals so that PL and PR transcripts extend into genes such as red, O and P necessary for the middle stage. The early and middle transcripts and patterns of expression therefore overlap. The cro product is sufficiently accumulated, it prevents transcription from PL and PR. The gene Q is expressed from the distal portion of the extended PR transcript and is responsible for the middle to late switch. This also operates the anti-termination. The Q product specifically antiterminates the short PR transcript extending it into the late genes, across the cohered cos region, so that many mature 4/14/12 phage particles are produced.
Phage vectors: There are two types of Phage vectors, viz: insertional and replacement vectors. Wild type Phage contains several sites for the restriction endonucleases and therefore is not suitable as a vector. However, derivatives of Phage produced by either insertion or deletion of phage genes are being used as vectors. Phage that have a single target site at which foreign DNA can be inserted (insertional vectors) or have a pair of sites defining a fragment that can be removed (stuffer) and replaced by foreign DNA (replacement vectors). A normal phage can accommodate only 5% more than its normal complement of DNA, vector derivatives are constructed with deletions to increase the space within the genome. The shortest DNA molecules that produce normal size plaques are 25% deleted. 4/14/12 If too-much non-essential DNA is deleted from the genome, it
This can be of an advantage to positively select recombinant phage carrying foreign DNA. If replaceable fragment of the replacement vector is either removed by physical separation or effectively destroyed by treatment with a second restriction endonuclease (that cuts it alone), then the deleted vector genome can give rise to plaques only if a new DNA segment is inserted into it. Improved properties of phage vectors: Aims for improvisation of phage vectors; 1. To increase the capacity for foreign DNA fragments, preferable generated by several RE 2. To devise methods for positively selecting recombinant formation 3. To allow RNA probes to be conveniently prepared by transcription of the foreign DNA insert; this facilitates the screening of libraries in chromosome walking procedures, eg: ZAP 4. To develop vectors for the insertion of eukaryotic cDNA such that expression of the cDNA, in the form of a fusion polypeptide with galactosidase, is driven in E.coli; this form of expression vector is useful in antibody screening. Eg: gt11. 4/14/12
Wild type cannot grow on E.coli strains lyosogenic for phage P2, ie the phage is Spi+ (sensitive to P2 inhibition). It has been observed that the products of red and gam genes of phage (which lie in the region 64% to 69%) are responsible for the inhibition of growth in a P2 lysogen. Hence vectors have been derived in which the stuffer fragment includes the region 64% to 69% , so that the recombinants in which this has been replaced by foreign DNA are phenotypically Spi- and can be positively selected by plating on a P2 lysogen. The gam gene product is necessary for the normal switch in DNA replication from bidirectional mode to the rolling circle mode. Gam- phage cannot generate the concatemeric linear DNA which is normally packed into the phage heads. However, gam- phage do form plaques because the rec and red recombination systems act on circular DNA molecules to form multimers, which can be packed. gam- red- phage are totally dependent on the rec-mediated exchange for plaque formation on rec+ bacteria. DNA 4/14/12 is a poor substrate for this rec-mediated exchange.
Therefore, such phage make vanishingly small plaques unless they contain one or more short DNA sequences called chi sites (cross over hot-spot instigator), which stimulate rec-mediated exchange. Many of the replacement vectors generate red- gam- clones and so have been constructed with a chi site within the non-replaceable part of the phage. The most recent generation of vectors, which are based on EMBL3 and EMBL4, have the capacity for DNA of size 9-23 kb. They are chi+ and also have polylinkers flanking the stuffer fragment to facilitate library construction. Phages with inserts can be selected on the basis of their Spiphenotype, but there is also an alternative. The vector can be digested with BamHI and EcoRI prior to ligation with foreign DNA fragments produced with BamHI. If the small BamHI-EcoRI fragments from the polylinkers are removed, the stuffer fragment will not be reincorporated.
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The structure of bacteriophage cloning vectors EMBL3 and EMBL4. The polylinker sequence is present in opposite orientation in the two vectors. 4/14/12
In the presence of phage head precursor (geneE pdt, major capsid) and the pdt of gene A, the concaemeric DNA is cleaved into monomers and encapsidated. Nicks are introduced in opposite strands of the DNA, 12 nucleotide pairs apart at each cos site, to produce the linear monomer with its cohesive termini. The pdt of geneD is then incorporated into what now becomes a complete phage head. The pdts of genes W and FII, among others then unite the head with a separately assembled tail structure to form the mature particle.
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In vitro packing of phage DNA: The principle of in vitro packing of phage DNA is to supply the ligated recombinant DNA with high concentrations of phage head precursor, packaging proteins, and phage tails. This is most efficiently performed in a very concentrated mixed lysate of two induced lysogens, One of which is blocked at the pre-head stage by an amber mutation in gene D and therefore accumulates this precursor, While the other is prevented from forming any head structure by an amber mutation in gene E. In the mixed lysate , genetic complementation occurs and exogenous DNA is packaged. Although concatemeric DNA is the substrate for packaging (covalently package added monomeric DNA, which presumably first concatemerizes non-covalently. 4/14/12
joined concatemers are, of course, produced in the ligation reaction by association of the natural cohesive ends of ), the in vitro system will
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DNA cloning with single-stranded DNA vectors: M13, f1 and fd are filamentous coliphages containing a circular single-stranded DNA molecule. Unique properties of filamentous bacteriophage: The filamentous bacteriophage contain a single-stranded circular DNA molecule which is 6404 (M13) or 6408 (fd) nucleotides long. The nucleotide sequence of these is 97% identical and the differences consist of the isolated nucleotides , mostly affecting the redundant bases of codons, with no blocks of sequence divergence. These filamentous phage only infect the enteric bacteria harboring F pili. The adsorption site appears to be the end of the F pilus. Replication of the phage DNA does not result in cell lysis. Rather the infected cells continue to grow and divide, though at a smaller rate than the non infected cells. Approx. 1000 phage particles are extruded from the cell into the medium per generation. 4/14/12
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The singlestranded DNA phage enters the cell by a process in which the decapsidation and replication are tightly coupled. The capsid proteins enter the cytoplasmic membrane as the viral DNA passes into the cell while being converted to a double stranded replicative form (RF). The RF multiplies rapidly until about 100 RF molecules are formed inside the cell. Replication of the RF then becomes asymmetric, due to the accumulation of a viral-encoded single-stranded specific DNAbinding protein. This protein binds to the viral strand and prevents synthesis of the complementary strand. From this point, only viral single strands are synthesized. These progeny single strands are released from the cell as filamentous particles following morphogenesis at the cell membrane. As the DNA passes through the membrane, the DNA-binding protein is stripped off and replaced by capsid protein. 4/14/12
Uses of vectors with ss-DNA genomes: As ss vectors, the filamentous phage have a number of advantages.
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The phage DNA is replicated via a double stranded circular DNA (RF) intermediate. This RF can be purified and manipulated in vitro just like a plasmid. Both RF and the ss-DNA will transfected competent E.coli cells to yield either plaques or infected colonies, depending on the assay method. The size of the phage particle is governed by the size of the viral DNA and therefore there are no packaging constraints. Indeed viral DNA upto six times the length of the M13 DNA has been packaged. With these phages it is very easy to determine the orientation of an insert. (although the relative orientation can be
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determined from restriction analysis of RF, there is an easier method. If two clones carry the insert in opposite directions, the ss-DNA from them will hybridize and this can be detected by agarose gel electrophoresis. Phage from 4/14/12 as little as 0.1ml of culture can be used in assays of this sort, making mass screening of cultures easy).
Modification of M13 for a better vector: The filamentous phage do not have any non-essential genes which can be used as cloning sites. In M13 there are 507 bp intergenic region, which contains the origins of DNA replication for both viral and the complementary strands. In most of the vectors developed so far foreign DNA has been inserted at this site. The wild type phage are not very promising since they contain very few unique sites within the intergenic region: AsuI in fd and AsuI and AvaI in M13. In the first example of M13 cloning, RF was partially digested with the BsuI and linear full length molecules were isolated by AGE. These linear monomers were blunt end ligated to a HindII restriction fragment comprising of the E.coli lac regulatory region and the genetic information for the -peptide of the galactosidase. The complete ligation mixture was used to transform a strain of E.coli with a deletion of the -galactosidase 4/14/12 peptide. The recombinant phage was detected by intergeneic
Insertion of DNA fragments into the lac region of M13mp1 destroys its ability to form blue plaques, making detection of recombinants easy. However, the lac region only contains unique sites for AvaII, Bg1I and PvuI and three sites for PvuII. It has no sites for the commonly used EcoRI or HindIII. To remedy this, mutagenesis of a single change in the base pair was done to create unique site for EcoRI within the lac fragment. This variant was designated as M13mp2. This phage was further modified to generate derivatives with polylinkers upstream of the lac -fragment. These derivatives (mp7-mp11, mp18, mp19) are the exact M13 counterparts of the pUC plasmids.
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Restriction map of cloning vector M13mp18. Phages M13mp18 and M13mp19 are 7249 bases in length and differ only in the orientation of the 54- bases polylinker that they carry. The map shows the restriction sites of enzymes that cut the molecule once or twice. The unique sites are shown in bold type. 4/14/12
Phasmids: These are vectors which have combined elements from plasmids and phages or if they contain an M13 ori region, phagemids. A group of phasmids that is widely used is the ZAP series of vectors used for cDNA cloning. Many different features that facilitate cloning and expression can be found combined in a single vector. Purified vector DNA plus associated reagents can be purchased from molecular biology suppliers. Cloning larger pieces of DNA and manipulating genes are two general uses of cloning vectors. The larger the pieces of DNA, easier it is to construct the final picture. Larger fragments are also needed to walk along the genome to isolate a gene
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Vectors for cloning large fragments of DNA: Cosmids: Plasmids have been constructed which contain a fragment of DNA including the cos site. These plasmids are termed as cosmids and can be used as gene cloning vectors in conjunction with the in vitro packaging system. Packaging of cosmid recombinants into phage coats imposes a desirable selection upon their size. With a cosmid vector of 5kb, we can insert 32-47 kb of foreign DNA,,,,,,,,,, much more than a phage- vector can accommodate. After packaging in vitro, the phage particle is used to infect a suitable host. The recombinant cosmid DNA is injected and circularizes like phage DNA but replicates as a normal plasmid without the expression of any phage functions. Transformed cells are selected on the basis of a vector drug resistance marker. 4/14/12
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Cosmids provide an efficient means of cloning large pieces of foreign DNA and hence form attractive vectors for constructing libraries of eukaryotic genome fragments. Partial digestion with RE provides suitably large fragments. However, a potential problem associated with the use of these partial digests is the possibility of two or more genome fragments joining together in the ligation reaction, hence creating a clone containing fragments that were not initially adjacent in the genome. This would give an incorrect data about the chromosomal organization. The problem can be solved by dephosphorylating the foreign DNA fragments so as to prevent their ligation together. This method is very sensitive to the exact ratio of target-tovector DNAs, because vector-to-vector ligation can occur. Also, recombinants with duplicated vector are unstable and break down in the host by recombination, resulting in the propagation of a non-recombinant cosmid vector. 4/14/12
An alternative solution to these problems is the construction of the cosmid c2XB. This cosmid carries a BamHI insertion site and two cos sites separated by a blunt end restriction site. The creation of these blunt ends, which ligate only very inefficiently under the conditions used, effectively prevents vector self-ligation in the ligation reaction.
Modern cosmids of the pWE and sCos series contain features such as:
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Multiple cloning sites for simple cloning using non-sizeselected DNA Phage promoters flanking the cloning site and Unique NotI, SacII or SfiI sites (G+C RE sites) flanking the cloning site to permit removal of the insert from the vector as single fragments.
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BAC and PAC vectors: Phage P1 is a temperate phage of E.coli and can mediate generalized transduction. A P1 vector system has been developed which has a capacity for DNA fragments as large as 100kb. Thus the capacity is about twice that of cosmid clones, but less than that of yeast artificial chromosome(YAC) clones. The P1 vector contains a packaging site (pac) which is necessary for in vitro packaging of recombinant molecules into phage particles. The vectors contain two lox P sites, which are recognized by the phage recombinanse ( product of phage cre gene) and which lead to circularization of the packaged DNA after it has been injected into an E.coli host expressing the recombinase. The clones are maintained in E.coli as low copy number plasmids by selection for a vector kanamycin-resistance marker. A high copy number can be induced by exploitation of the P1 lytic replicon. 4/14/12
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Shizuya et al have developed a bacterial cloning system for mapping and analysis of complex genomes. This BAC system is based on the single-copy sex factor F of E.coli. This vector includes the cosN and P1 loxP sites, two cloning sites (HindIII and BamHI) and several G+C restriction enzyme sites for potential excision of the inserts. The cloning site is flanked by T7 and SP6 promoters for generating RNA probes. This BAC can be transformed into E.coli efficiently, thus avoiding the packaging extracts that are required with the P1 system. BACs are capable of maintaining human and plant genome fragments, greater than 300kb for over 100 generations with a high degree of stability. They have been used for constructing genomic libraries with an average insert size of 125kb.
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Structure of a BAC vector derived from a mini-F plasmid. The oriS and repE genes mediate the unidirectional replication of the F factor, while parA and parB maintain the copy number at a level of one or two per genome. CmR is a chloramphenicol marker. cosN and loxP are the cleavage sites for the treminase and P1 cre protein, espectively. HindIII and BamHI are unique cleavage sites for inserting foreign DNA.
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Two widely used BAC vectors, pBeloBAC11 and pECBAC1 have a lacZ gene with multiple cloning sites. pBeloBAC11 has two EcoRI sites, one in the lacZ gene and one in the CmR gene, whereas pECBAC1 has only the EcoRI site in the LacZ gene. Further improvement of BAC vectors was by including a site for the insertion of a transposon. This enables genomic inserts to be modified after cloning in bacteria, a procedure known as retrofitting.
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Recombinogenic engineering: This simplifies the cloning of DNA, particularly with highmolecular weight constructs. BACs or PACs are useful in cloning complete operons or large gene clusters. But subsequent engineering of clones is very difficult, due to two reasons: a. Very large plasmids are difficult to manipulate in vitro without shearing and if intact have a restricted mobility in gel electrophoresis.
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The longer the DNA insert the more likely it is to have multiple sites for each common RE.
Hence any cleavage and ligation could reduce the size of the DNA insert . To avoid these problems it is necessary to carry out the manipulations in vovo instead of in vitro by making use of homologous recombination. 4/14/12
Two variants of in vivo recombinogenic engineering. In both variations the target molecule remains intact and could be a BAC, PAC, any other plasmid, or the E.coli chromosome. a. replacement of a segment of a target molecule with linear DNA molecule that is introduced to the host cell of the plasmid by electroporation. b. Removal of the selectable gene by recombination at recombinase target sites. A and B : regions of homology (35-60nucleotides), sm : selectable marker, arrowhead : recombinase target site 4/14/12
A linear targeting DNA carrying short homology regions flanking a selectable gene is introduced by electroporation into cells carrying the BAC or PAC to be modified. In many cases the persistence of the selectable gene (sm) in the product is undesirable and hence a second round of recombinogenic engineering is required. In the first round, an initial product is formed by integration of the selectable gene, together with additional functional elements. In the second round, the extra functional elements are used to remove selectable genes, thereby generating the final product.
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Specialist-purpose vectors: M13 based vectors can be used to make single-stranded DNA suitable for sequencing
The more preferred vectors now are the pUC based phagemids which contain the M13 ori region as well as the pUC (ColE1) ori region.
Expression vectors enable a cloned gene to be placed under control of a promoter that functions in E.coli.
Expression vectors are required if one wants to prepare RNA probes from the cloned gene or to purify large amounts of the gene product. Transcription of the cloned gene is required, generally under the promoter specific for the vector. Such vector carried promoters are optimized for binding of E.coli RNA polymerase and many of them can be regulated easily by changes in the growth conditions.
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Specialists vectors have been developed that facilitate the production of RNA probes and interfering RNA.
This is because RNA-DNA hybridization is more stable than the DNA-DNA hybridization. Hence RNA probes are constructed by cloning the relevant gene sequence in a plasmid vector that is under the control of a phage promoter. After the purification the plasmid is linearized with a suitable RE and then incubated with phage RNA polymerase and four ribonucleotides.. No transcription terminator is required because the RNA polymerase will fall off at the end of the linearized plasmid. Phage promoters are used for three reasons: a. Such promoters are very strong, enabling large amounts of RNA to be made in vitro. b. The phage promoter is not recognized by the E.coli RNA polymerase and so no transcription will occur inside the cell. c. The RNA polymerase encoded by phage such as SP6, T7 and T3 are much simpler molecules to handle than E.coli enzyme.
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Method for preparing RNA probes from cloned DNA molecule using a phage SP6 promoter and SP6 RNA polymerase. 4/14/12
If it is planned to probe RNA or single-stranded DNA sequences, then it is essential to prepare RNA probes corresponding to both strands of the insert. One way of doing this is to have two different clones corresponding to the two orientations of the insert. An alternative method is to use a cloning vector in which the insert is placed between two different opposing phage promoters that flank a multiple cloning sequence. Since each of the two promoters is recognized by a different RNA polymerase, the direction of transcription is determined by which polymerase is used. Further improvement was using LITMUS vectors, in which polylinker regions are flanked by two modified T7 RNA polymerase promoters.
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Structure and use of LITMUS vectors for making RNA probes. a. Structure of the LITMUS vector showing the orientation and restriction sites of the four polylinkers b. Method of using the LITMUS vectors to selectively synthesize RNA probes from each strand of a cloned insert.
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RNAi: This is a RNA dependent gene silencing process that is controlled by the RNA-induced silencing complex (RISC) and is initiated by short ds-RNA molecules. An enzyme dicer cleaves the long ds-RNA molecules into short fragments of approx 20bps. One of the strands is known as guide strand. This is incorporated into the RNA-induced silencing complex. The most studied outcome of RNAi is the post transcriptional gene silencing. Here the guide strand base pairs with a complementary sequence of a messenger RNA molecule and induces cleavage by Argonaute (catalytic protein component of RISC).
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Vectors with strong, controllable promoters are used to maximize synthesis of cloned gene products.
If the cloned gene is preceded by a promoter recognized by the host cell, there is a high probability that there will be detectable synthesis of the cloned gene product. However, due to commercial requirements, if large quantities of proteins are required then this expression needs to be maximized. There are several factors that affect the expression of the cloned genes. Viz: promoter strength, transcriptional termination, plasmid copy number, plasmid stability, host cell physiology, mRNA structure, etc. While using a strong promoter, the effects of overexpression are also to be considered. Many gene products can be toxic to the host cell even when synthesized in small amounts. Eg: surface proteins. Even when overexpression of a protein is not toxic to the host cell, high-level synthesis exerts a metabolic drain on the cell.
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This leads to slower growth and hence in culture there is selection for variants with lower or no expression of the cloned gene because these will grow faster. To minimize the problems associated with high-level expression, the vector selected is such in which the cloned gene is under the control of a regulated promoter. Different vectors have been constructed for regulated expression of gene inserts. Eg: PL, T7, trc (tac) or BAD. The trc and tac promoters are hybrid promoters derived from the lac and trp promoters. They are stronger than the parental promoters. Like lac, the trc and tac promoters are inducible by lactose and IPTG. The vectors using these promoters also carry the lacO operator and the lacI gene which encodes the repressor.
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Strategy for regulating the expression of genes cloned into a pET vector. The gene for T7 RNA polymerase (gene1) is inserted into the chromosome of E.coli and transcribed from the lac promoter. Hence it is expressed only when the inducer IPTG is added. The T7 RNA polymerase will then transcribe the gene cloned into the pET vector. If the protein product is toxic, the transcription can be reduced before induction. The T7 lysozyme encoded by a compatible plasmid, pLysS, will bind to any residual T7 RNA polymerase made in absence of inducer 4/14/12 and inactivate it. Also, the presence of lac operators between the T7 promoter
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Three different examples of tags are: a. Polyhistidine fusion for purification..enterokinase cleavage site
Structure of a vector (pBAD/His) designed for the expression of a cloned gene as a fusion protein containing a polyhistidine sequence. Three different varients allow the insert to be placed in each of the three translational reading frames. The sequence shaded purple shows the base sequence which is altered in each of the three vectors. The lightly shaded box (AGATCT) is the Bgl II site of the polylinker. The gene of interest is engineered into a vector in which there is a polylinker downstream of six histidine residues and a proteolytic cleavage site for enterokinase. After induction of synthesis of the fusion protein, the cells are lysed and the lysate is applied on to a column containing immobilized divalent Nickel, which selectively binds the polyhistidine tag. After washing away any contaminating proteins, the fusion protein is eluted from the column and treated with enterokinase
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b. Short antibody recognition sequences can be incorporated into the tag between the affinity label and the protease cleavage site. These antibodies can be used to detect, fusion proteins carrying the appropriate epitope. c. Biotin tags can be used for purification of the expressed protein using affinity chromatography. Streptavidin has a strong affinity for Biotin and the biotin-streptavidin interaction is considered as the strongest amongst the noncovalent biological interaction. The disadvantage of the affinity purification system is that a. a protease is required to separate the target protein from the affinity tag. b. Also the protease has to be separated from the protein of interest. Modification was done to this method by introducing a protein splicing element, an intein gene, that undergoes a self cleavage at low temperature at its N terminus in presence of thiols like cysteine, dithiothreitol or -mercaptoethanol. The vector construct is placed under the control of an IPTG-inducible T7 promoter. 4/14/12
Purification of a cloned gene product synthesized as a fusion to the biotin carboxylase carrier protein (tag).
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Vectors that promote solubilization of expressed proteins Overproduction of proteins in E.coli leads to sequestration of the product into soluble aggregates or inclusion bodies. Lowering of growth temperature has reported increase in yield of the correctly folded soluble protein. Media components and pH values that lower the growth rate also reduce the inclusion body formation. Three methods have been described to prevent inclusion body formation. a. The host cell is engineered to overproduce a chaperon (proteins whose function is to assist with the folding and refolding of other proteins), in addition to the protein of interest. b. Making minor changes to the amino acid sequence of the target protein, eg: cysteine to serine change in fibroblast growth factor minimized inclusion body formation. c. It is derived from the observation that many proteins produced as insoluble aggregates in their native state are synthesized in 4/14/12 soluble form as thioredoxin fusion proteins. Also NusA, GrpE and
Proteins that are synthesized with signal sequences are exported from the cell Proteins secreted in the cytoplasm are released into the periplasm or intergrated into or transported across the outer membrane. The proteins are exported through the inner membrane to the periplasm or to the outer membrane by a general export pathway (GEP). The proteins that enter the GEP are synthesized in the cytoplasm with a signal sequence at the N terminus. This sequence is cleaved by a signal or leader peptidase during transport. A signal sequence has three domains: A positively charged amino-terminal region, a hydrophobic core (515 hydrophobic aas) and a leader peptidase cleavage site. A signal sequence attached to a normally cytoplasmic protein directs it to the export pathway.
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The Gateway system is a highly efficient method for transferring DNA fragments to a large number of different vectors The Gateway system is designed to replace all the steps involving restriction enzymes to a simple two step procedure.
The principle of Gateway system: following transformation, the only cells that can form colonies are ones carrying plasmid encoding ApR and lacking ccdB ( counterselectable marker) 4/14/12
The use of Gateway system to move a gene unchanged from an entry clone to many different vectors. 4/14/12