WO2005040377A2 - High efficiency gene transfer and expression in mammalian cells by a multiple transfection procedure of matrix attachment region sequences - Google Patents
High efficiency gene transfer and expression in mammalian cells by a multiple transfection procedure of matrix attachment region sequences Download PDFInfo
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Definitions
- the present invention relates to purified and isolated DNA sequences having protein production increasing activity and more specifically to the use of matrix attachment regions (MARs) for increasing protein production activity in a eukaryotic cell. Also disclosed is a method for the identification of said active regions, in particular MAR nucleotide sequences, and the use of these characterized active MAR sequences in a new multiple transfection method.
- MARs matrix attachment regions
- BACKGROUND OF THE INVENTION nowadays, the model of loop domain organization of eukaryotic chromosomes is well accepted (Boulikas T, "Nature of DNA sequences at the attachment regions of genes to the nuclear matrix", J. Cell Biochem., 52:14-22, 1993).
- chromatin is organized in loops that span 50-100 kb attached to the nuclear matrix, a proteinaceous network made up of RNPs and other nonhistone proteins (Bode J, Stengert-lber M, Kay V, Schalke T and Dietz-Pfeilstetter A, Crit. Rev. Euk. Gene Exp., 6:115-138, 1996).
- SAR DNA regions attached to the nuclear matrix
- MAR DNA regions attached to the nuclear matrix
- these regions may define boundaries of independent chromatin domains, such that only the encompassing cis-regulatory elements control the expression of the genes within the domain.
- MAR elements can enhance expression of heterologous genes in cell culture lines (Kalos M and Fournier R (1995) "Position-independent transgene expression mediated by boundary elements from the apolipoprotein B chromatin domain" Mol Cell Biol 15,198-207), transgenic mice (Castilla J, Pintado B, Sola, I, Sanchez-Morgado J, and Enjuanes L (1998) "Engineering passive immunity in transgenic mice secreting virus-neutralizing antibodies in milk” Nat Biotechnol 16, 349- 354) and plants (Allen G, Hall GJ, Michalowski S, Newman W, Spiker S, Weissinger A, and Thompson W (1996), "High-level transgene expression in plant cells: effects of a strong scaffold attachment region from tobacco" Plant Cell 8, 899-913).
- chromatin-structure modifying sequences including MARs as exemplified by the chicken lysozyme 5' MAR is able to significantly enhance reporter expression in pools of stable Chinese Hamster Ovary (CHO) cells (Zahn-Zabal M, et al., "Development of stable cell lines for production or regulated expression using matrix attachment regions” J Biotechnol, 2001 , 87(1): p. 29-42). This property was used to increase the proportion of high-producing clones, thus reducing the number of clones that need to be screened.
- this technique does not generate a homogenous population of transfected cells, since it cannot favour the integration of further gene copy, nor does it direct the transgenes to favorable chromosomal loci, ii) the use of the same selectable marker in multiple transfection events does not permit the selection of doubly or triply transfected cells.
- MAR-Finder http://futuresoft.org/MarFinder; Singh GB, Kramer JA and Krawetz SA, "Mathematical model to predict regions of chromatin attachment to the nuclear matrix", Nucleic Acid Research, 25:1419-1425, 1997) is based on set of patterns identified within several MARs and a statistical analysis of the co-occurrence of these patterns. MAR-Finder predictions are dependent of the sequence context, meaning that predicted MARs depend on the context of the submitted sequence. The other predictive software, SMARTest (http://www.
- SMARTest is said to be suitable to perform large-scale analyses. But actually aside its relative poor specificity, the amount of hypothetical MARs rapidly gets huge when doing large scale analyses with it, and in having no way to increase its specificity to restrain the number of hypothetical MARs, SMARTest becomes almost useless to screen for potent MARs form large DNA sequences.
- the object of this invention is to 1) understand the functional features of MARs that allow improved recombinant protein expression; 2) get a new Bioinformatic tool compiling MAR structural features as a prediction of function, in order to 3) perform large scale analyses of genomes to identify novel and more potent MARs, and, finally 4) to demonstrate improved efficiency to increase the production of recombinant proteins from eukaryotic cells or organisms when using the newly identified MAR sequences.
- Fig. 1 shows the distribution plots of MARs and non-MARs sequences. Histograms are density plots (relative frequency divided by the bin width) relative to the score of the observed parameter. The density histogram for human MARs in the SMARt DB database is shown in black, while the density histogram for the human chromosome 22 are in grey.
- Fig. 2 shows Scatterplots of the four different criteria used by SMAR Scan® and the AT-content with human MARs from SMARt DB.
- Fig. 3 shows the distribution plots of MAR sequences by organism. MAR sequences from SMARt DB of other organisms were retrieved and analyzed. The MAR sequences density distributions for the mouse, the chicken, the sorghum bicolor and the human are plotted jointly.
- Fig. 4 shows SMAR Scan® predictions on human chromosome 22 and on shuffled chromosome 22.
- Top plot Average number of hits obtained by SMAR Scan® with five: rubbled, scrambled, shuffled within nonoverlapping windows of 10 bp, order 1 Markov chains model and with the native chromosome 22.
- Bottom plot Average number of MARs predicted by SMAR Scan® in five: rubbled, scrambled, shuffled within non- overlapping windows of 10 bp, order 1 Markov chains model and with the native chromosome 22.
- Fig. 5 shows the dissection of the ability of the chicken lysozyme gene 5'-MAR to stimulate transgene expression in CHO-DG44 cells. Fragments B, K and F show the highest ability to stimulate transgene expression. The indicated relative strength of the elements was based on the number of high-expressor cells.
- Fig. 6 shows the effect of serial-deletions of the 5'-end (upper part) and the 3'-end (lower part) of the 5'-MAR on the loss of ability to stimulate transgene expression.
- the transition from increased to decreased activity coincide with B-, K- and F-fragments.
- Fig. 7 shows that portions of the F fragment significantly stimulate transgene expression.
- the F fragment regions indicated by the light grey arrow were multimerized, inserted in pGEGFP Control and transfected in CHO cells.
- the element that displays the highest activity is located in the central part of the element and corresponds to fragment FIN (black bar labelled minimal MAR).
- an enhancer activity is located in the 3'-flanking part of the Fill fragment (dark grey bar labelled MAR enhancer).
- Fig. 8 shows a map of locations for various DNA sequence motifs within the cLysMAR.
- Fig. 8 (B) represents a Map of locations for various DNA sequence motifs within the cLysMAR.
- Vertical lines represent the position of the computer-predicted sites or sequence motifs along the 3034 base pairs of the cLysMAR and its active regions, as presented in Fig. 5.
- the putative transcription factor sites, (MEF2 05, Oct-1 , USF-02, GATA, NFAT) for activators and (CDP, SATB1 , CTCF, ARBP/MeCP2) for repressors of transcription, were identified using Matlnspector (Genomatix), and CpG islands were identifed with CPGPLOT.
- Motifs previously associated with MAR elements are labelled in black and include CpG dinucleotides and CpG islands, unwinding motifs (AATATATT and AATATT), poly As and Ts, poly Gs and Cs, Drosophila topoisomerase II binding sites (GTNWAYATTNATTNATNNR) which had identity to the 6 bp core and High mobility group I (HMG-I/Y) protein binding sites.
- Other structural motifs include nucleosome-binding and nucleosome disfavouring sites and a motif thought to relieve the superhelical strand of DNA.
- Fig. 8(A) represents the comparison of the ability of portions of the cLysMAR to activate transcription with MAR prediction score profiles with MarFinder.
- the top diagram shows the MAR fragment activity as in Fig. 5, while the middle and bottom curves show MARFinder-predicted potential for MAR activity and for bent DNA structures respectively.
- Fig. 9 shows the correlation of DNA physico-chemical properties with MAR activity.
- Fig. 9(A) represents the DNA melting temperature, double helix bending, major groove depth and minor groove width profiles of the 5'-MAR and were determined using the algorithms of Levitsky et al (Levitsky VG, Ponomarenko MP, Ponomarenko JV, Frolov AS, Kolchanov NA "Nucleosomal DNA property database", Bioinformatics, 15; 582592, 1999).
- the most active B, K and F fragments depicted at the top are as shown as in Figure 1.
- Fig. 9(A) represents the DNA melting temperature, double helix bending, major groove depth and minor groove width profiles of the 5'-MAR and were determined using the algorithms of Levitsky et al (Levitsky VG, Ponomarenko MP, Ponomarenko JV, Frolov AS, Kolchanov NA "Nucleosomal DNA property database", Bioinformatics, 15; 582592, 1999).
- FIG. 9(B) represents the enlargement of the data presented in panel A to display the F fragment map aligned with the tracings corresponding to the melting temperature (top curve) and DNA bending (bottom curve). The position of the most active FIB fragment and protein binding site for specific transcription factors are as indicated.
- Fig. 10 shows the distribution of putative transcription factor binding sites within the 5'- cLysMAR. Large arrows indicate the position of the CUE elements as identified with SMAR Scan®.
- Fig. 11 shows the scheme of assembly of various portions of the MAR.
- the indicated portions of the cLysMAR were amplified by PCR, introducing Bglll-BamHI linker elements at each extremity, and assembled to generate the depicted composite elements.
- the top construct consists of the assembly of all CUE and flanking sequences at their original location except that Bgll-BamHII linker sequences separate each element.
- Fig. 12 represents the plasmid maps.
- Fig. 13 shows the effect of re-transfecting primary transfectants on GFP expression.
- Cells (CHO-DG44) were co-transfected with pSV40EGFP (left tube) or pMAR- SV40EGFP (central tube) and pSVneo as resistance plasmid.
- Cells transfected with pMAR-SV40EGFP were re-transf ected 24 hours later with the same plasmid and a different selection plasmid, pSVpuro (right tube). After two weeks selection, the phenotype of the stably transfected cell population was analysed by FACS.
- Fig. 14 shows the effect of multiple load of MAR-containing plasmid.
- the pMAR- SV40EGFP/ pMAR-SV40EGFP secondary transfectants were used in a third cycle of transfection at the end of the selection process.
- the tertiary transfection was accomplished with pMAR or pMAR-SV40EGFP to give tertiary transfectants. After 24 hours, cells were transfected again with either plasmid, resulting in the quaternary transfectants (see Table 4).
- Fig. 15 shows comparative performance of SMAR prediction algorithms exemplified by region WP18A10A7.
- SMAR Scan® analysis was performed with default settings.
- SIDD analysis top curve and left-hand side scale
- the attachment of several DNA fragments to the nuclear matrix in vitro was taken from Goetze et al ( Goetze S, Gluch A, Benham C, Bode J, "Computational and in vitro analysis of destabilized DNA regions in the interferon gene cluster: potential of predicting functional gene domains.” Biochemistry, 42:154-166, 2003).
- Fig. 16 represents the results of a a gene therapy-like protocol using MARs.
- Fig. 17 represents the scatterplot for the 1757 S/MAR sequences of the AT (top) and TA (bottom) dinucleotide percentages versus the predicted DNA bending as computed by SMAR Scan®.
- Fig. 18 represents the dinucleotide percentage distribution plots over the 1757 non- S/MARs sequences.
- Fig.19 shows the effect of various S/MAR elements on the production of recombinant green fluorescent protein (GFP).
- GFP green fluorescent protein
- Fig. 20 depicts the effect of the induction of hematocrit in mice injected by MAR- network.
- the present invention relates to a purified and isolated DNA sequence having protein production increasing activity characterized in that said DNA sequence comprises at least one bent DNA element, and at least one binding site for a DNA binding protein.
- Certain sequences of DNA are known to form a relatively "static curve", where the DNA follows a particular 3-dimensional path.
- the piece of DNA can form a flat, planar curve also defined as bent DNA (Marini, et al., 1982 "Bent helical structure in kinetoplast DNA”, Proc. Natl. Acad. Sci. USA, 79: 7664-7664).
- the bent DNA element of a purified and isolated DNA sequence having protein production increasing activity of the present invention usually contains at least 10% of dinucleotide TA, and/or at least 12% of dinucleotide AT on a stretch of 100 contiguous base pairs.
- the bent DNA element contains at least 33% of dinucleotide TA, and/or at least 33% of dinucleotide AT on a stretch of 100 contiguous base pairs.
- the purified and isolated DNA sequence usually comprises a MAR nucleotide sequence selected from the group comprising the sequences SEQ ID Nos 1 to 27 or a cLysMAR element or a fragment thereof.
- the purified and isolated DNA sequence is a MAR nucleotide sequence selected from the group comprising the sequences SEQ ID Nos 1 to 27, more preferably the sequences SEQ ID Nos 24 to 27.
- Encompassed by the present invention are as well complementary sequences of the above-mentioned sequences SEQ ID Nos 1 to 27 and the cLysMAR element or fragment, which can be produced by using PCR or other means.
- An “element” is a conserved nucleotide sequences that bears common functional properties (i.e. binding sites for transcription factors) or structural (i.e. bent DNA sequence) features.
- a part of sequences SEQ ID Nos 1 to 27 and the cLysMAR element or fragment refers to sequences sharing at least 70% nucleotides in length with the respective sequence of the SEQ ID Nos 1 to 27. These sequences can be used as long as they exhibit the same properties as the native sequence from which they derive. Preferably these sequences share more than 80%, in particular more than 90% nucleotides in length with the respective sequence of the SEQ ID Nos 1 to 27.
- the present invention also includes variants of the aforementioned sequences SEQ ID Nos 1 to 27 and the cLysMAR element or fragment, that is nucleotide sequences that vary from the reference sequence by conservative nucleotide substitutions, whereby one or more nucleotides are substituted by another with same characteristics.
- sequences SEQ ID Nos 1 to 23 have been identified by scanning human chromosome 1 and 2 using SMAR Scan®, showing that the identification of novel MAR sequences is feasible using the tools reported thereafter whereas SEQ ID No 24 to 27 have been identified by scanning the complete human genome using the combined SMAR Scan® method.
- the complete chromosome 1 and 2 were screened to identify bent DNA element as region corresponding to the highest bent, major groove depth, minor groove width and lowest melting temperature as shown in figure 3.
- this collection of sequence was scanned for binding sites of regulatory proteins such as SATB1 , GATA, etc. as shown in the figure 8B) yielding sequences SEQ ID 1-23.
- sequences 21-23 were further shown to be located next to known gene from the Human Genome Data Base.
- molecular chimera of MAR sequences are also considered in the present invention.
- molecular chimera is intended a nucleotide sequence that may include a functional portion of a MAR element and that will be obtained by molecular biology methods known by those skilled in the art.
- MAR elements particularly combinations of MAR elements or fragments or sub-portions thereof are also considered in the present invention.
- These fragments can be prepared by a variety of methods known in the art. These methods include, but are not limited to, digestion with restriction enzymes and recovery of the fragments, chemical synthesis or polymerase chain reactions (PCR).
- cLysMAR elements or fragments are also envisioned in the present invention, depending on the functional results to be obtained.
- Elements of the cLysMAR are e.g. the B, K and F regions as described in WO 02/074969, the disclosure of which is hereby incorporated herein by reference, in its entirety.
- the preferred elements of the cLysMAR used in the present invention are the B, K and F regions. Only one element might be used or multiple copies of the same or distinct elements (multimerized elements) might be used (see Fig. 8 A)).
- fragment is intended a portion of the respective nucleotide sequence.
- Fragments of a MAR nucleotide sequence may retain biological activity and hence bind to purified nuclear matrices and/or alter the expression patterns of coding sequences operably linked to a promoter.
- Fragments of a MAR nucleotide sequence may range from at least about 100 to 1000 bp, preferably from about 200 to 700 bp, more preferably from about 300 to 500 bp nucleotides.
- any combinations of fragments which have the same number of nucleotides present in a synthetic MAR sequence consisting of natural MAR element and/or fragments.
- the fragments are preferably assembled by linker sequences.
- Preferred linkers are Bglll-BamHI linker.
- Protein production increasing activity refers to an activity of the purified and isolated DNA sequence defined as follows: after having been introduced under suitable conditions into a eukaryotic host cell, the sequence is capable of increasing protein production levels in cell culture as compared to a culture of cell transfected without said DNA sequence. Usually the increase is 1.5 to 10 fold, preferably 4 to 10 fold. This corresponds to a production rate or a specific cellular productivity of at least 10 pg per cell per day (see Example 11 and Fig.13).
- Chromatin is the protein and nucleic acid material constituting the chromosomes of a eukaryotic cell, and refers to DNA, RNA and associated proteins.
- a "chromatin element” means a nucleic acid sequence on a chromosome having the property to modify the chromatine structure when integrated into that chromosome.
- Cross refers to the placement of two or more elements (such as chromatin elements) on the same nucleic acid molecule (such as the same vector, plasmid or chromosome).
- Trans refers to the placement of two or more elements (such as chromatin elements) on two or more different nucleic acid molecules (such as on two vectors or two chromosomes).
- Chromatin modifying elements that are potentially capable of overcoming position effects, and hence are of interest for the development of stable cell lines, include boundary elements (BEs), matrix attachment regions (MARs), locus control regions (LCRs), and universal chromatin opening elements (UCOEs).
- BEs boundary elements
- MARs matrix attachment regions
- LCRs locus control regions
- UOEs universal chromatin opening elements
- Boundary elements or insulator elements, define boundaries in chromatin in many cases (Bell A and Felsenfeld G. 1999; “Stopped at the border: boundaries and insulators, Curr Opin Genet Dev 9, 191-198) and may play a role in defining a transcriptional domain in vivo. BEs lack intrinsic promoter/enhancer activity, but rather are thought to protect genes from the transcriptional influence of regulatory elements in the surrounding chromatin.
- the enhancer-block assay is commonly used to identify insulator elements. In this assay, the chromatin element is placed between an enhancer and a promoter, and enhancer-activated transcription is measured. Boundary elements have been shown to be able to protect stably transfected reporter genes against position effects in Drosophila, yeast and in mammalian cells. They have also been shown to increase the proportion of transgenic mice with inducible transgene expression.
- Locus control regions are cis-regulatory elements required for the initial chromatin activation of a locus and subsequent gene transcription in their native locations (Grosveld, F. 1999, "Activation by locus control regions?" Curr Opin Genet Dev 9, 152-157).
- the activating function of LCRs also allows the expression of a coupled transgene in the appropriate tissue in transgenic mice, irrespective of the site of integration in the host genome. While LCRs generally confer tissue-specific levels of expression on linked genes, efficient expression in nearly all tissues in transgenic mice has been reported for a truncated human T-cell receptor LCR and a rat LAP LCR. The most extensively characterized LCR is that of the globin locus. Its use in vectors for the gene therapy of sickle cell disease and (3-thalassemias is currently being evaluated.
- MARs may mediate the anchorage of specific DNA sequence to the nuclear matrix, generating chromatin loop domains that extend outwards from the heterochromatin cores. While MARs do not contain any obvious consensus or recognizable sequence, their most consistent feature appears to be an overall high A/T content, and C bases predominating on one strand (Bode J, Schlake T, RiosRamirez M, Mielke C, Stengart M, Kay V and KlehrWirth D, "Scaffold/matrix- attached regions: structural propreties creating transcriptionally active loci” structural and Functional Organization of the Nuclear Matrix: International Review of Citology, 162A:389453, 1995).
- BURs base- unpairing regions
- CUE core-unwinding element
- AATAAAYAAA AATAAAYAAA
- TWTWTTWTT T-box
- DNA unwinding motifs AATATATT, AATATT
- SATB1 binding sites H-box, A/T/C25
- consensus Topoisomerase II sites for vertebrates RNYNNCNNGYNGKTNYNY
- Drosophila GTNWAYATTNATNNR
- Ubiquitous chromatin opening elements (UCOEs", also known as “ubiquitously-acting chromatin opening elements") have been reported in WO 00/05393.
- an “enhancer” is a nucleotide sequence that acts to potentiate the transcription of genes independent of the identity of the gene, the position of the sequence in relation to the gene, or the orientation of the sequence.
- the vectors of the present invention optionally include enhancers.
- a “gene” is a deoxyribonucleotide (DNA) sequence coding for a given mature protein.
- the term “gene” shall not include untranslated flanking regions such as RNA transcription initiation signals, polyadenylation addition sites, promoters or enhancers.
- a “product gene” is a gene that encodes a protein product having desirable characteristics such as diagnostic or therapeutic utility.
- a product gene includes, e. g., structural genes and regulatory genes.
- a “structural gene” refers to a gene that encodes a structural protein.
- structural genes include but are not limited to, cytoskeletal proteins, extracellular matrix proteins, enzymes, nuclear pore proteins and nuclear scaffold proteins, ion channels and transporters, contractile proteins, and chaperones.
- Preferred structural genes encode for antibodies or antibody fragments.
- regulatory gene refers to a gene that encodes a regulatory protein.
- regulatory proteins include, but are not limited to, transcription factors, hormones, growth factors, cytokines, signal transduction molecules, oncogenes, proto-oncogenes, transmembrane receptors, and protein kinases.
- Orientation refers to the order of nucleotides in a given DNA sequence.
- an inverted orientation of a DNA sequence is one in which the 5' to 3' order of the sequence in relation to another sequence is reversed when compared to a point of reference in the DNA from which the sequence was obtained.
- reference points can include the direction of transcription of other specified DNA sequences in the source DNA and/or the origin of replication of replicable vectors containing the sequence.
- Eukaryotic cell refers to any mammalian or non-mammalian cell from a eukaryotic organism.
- any eukaryotic cell that is capable of being maintained under cell culture conditions and subsequently transfected would be included in this invention.
- Especially preferable cell types include, e. g., stem cells, embryonic stem cells, Chinese hamster ovary cells (CHO), COS, BHK21, NIH3T3, HeLa, C2C12, cancer cells, and primary differentiated or undifferentiated cells.
- Other suitable host cells are known to those skilled in the art.
- host cell and "recombinant host cell” are used interchangeably herein to indicate a eukaryotic cell into which one or more vectors of the invention have been introduced. It is understood that such terms refer not only to the particular subject cell but also to the progeny or potential progeny of such a cell. Because certain modifications may occur in succeeding generations due to either mutation or environmental influences, such progeny may not, in fact, be identical to the parent cell, but are still included within the scope of the term as used herein.
- introducing a purified DNA into a eukaryotic host cell denote any process wherein an extracellular DNA, with or without accompanying material, enters a host cell.
- cell transfected or “transfected cell” means the cell into which the extracellular DNA has been introduced and thus harbours the extracellular DNA.
- the DNA might be introduced into the cell so that the nucleic acid is replicable either as a chromosomal integrant or as an extra chromosomal element.
- Promoter refers to a nucleic acid sequence that regulates expression of a gene.
- Codon-transfection means the process of transfecting a eukaryotic cell with more than one exogenous gene, or vector, or plasmid, foreign to the cell, one of which may confer a selectable phenotype on the cell.
- the purified and isolated DNA sequence having protein production increasing activity also comprises, besides one or more bent DNA element, at least one binding site for a DNA binding protein.
- the DNA binding protein is a transcription factor.
- transcription factors are the group comprising the polyQpolyP domain proteins.
- transcription factor is a transcription factor selected from the group comprising SATB1 , NMP4, MEF2, S8, DLX1 , FREAC7, BRN2, GATA 1/3, TATA, Bright, MSX, AP1 , C/EBP, CREBP1 , FOX, Freac7, HFH1 , HNF3alpha, Nkx25, POU3F2, Pit1 , TTF1 , XFD1 , AR, C/EBPgamma, Cdc5, FOXD3, HFH3, HNF3 beta, MRF2, Oct1 , POU6F1 , SRF, V$MTATA_B, XFD2, Bach2, CDP CR3, Cdx2, FOXJ2, HFL, HP1 , Myc, PBX, Pax3, TEF, VBP, XFD3, Brn2, COMP1 , Evil, FOXP3, GATA4, HFN1 , Lhx3, NKX3A, POU1F1 , Pax
- SATB1 , NMP4 and MEF2 are known to regulate the development and/or tissue-specific gene expression in mammals. These transcription factors have the capacity to alter DNA geometry, and reciprocally, binding to DNA as an allosteric ligand modifies their structure.
- SATB1 was found to form a cage-like structure circumscribing heterochromatin (Cai S, Han HJ , and Kohwi-Shigematsu T, "Tissue- specific nuclear architecture and gene expression regulated by SATB1" Nat Genet, 2003. 34(1): p. 42-51).
- Yet another object of the present invention is to provide a purified and isolated cLysMAR element and/or fragment, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants. More preferably, the cLysMAR element and/or fragment are consisting of at least one nucleotide sequence selected from the B, K and F regions.
- a further object of the present invention is to provide a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences.
- the synthetic MAR sequence comprises a cLysMAR element and/or fragment a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- linker sequences are Bglll-BamHI linker.
- An other aspect of the invention is to provide a method for identifying a MAR sequence using a Bioinformatic tool comprising the computing of values of one or more DNA sequence features corresponding to DNA bending, major groove depth and minor groove width potentials and melting temperature.
- the identification of one or more DNA sequence features further comprises a further DNA sequence feature corresponding to binding sites for DNA binding proteins, which is also computed with this method.
- profiles or weight-matrices of said bioinformatic tool are based on dinucleotide recognition.
- the bioinformatic tool used for the present method is preferably, SMAR Scan®, which contains algorithms developed by Gene Express (http://srs6.bionet.nsc.ru/srs6bin/cgi- bin/wgetz?-e+[FEATURES-SitelD:'nR']) and based on Levitsky et al., 1999. These algorithms recognise profiles, based on dinucleotides weight-matrices, to compute the theoretical values for conformational and physicochemical properties of DNA.
- SMAR Scan® uses the four theoretical criteria also designated as DNA sequence features corresponding to DNA bending, major groove depth and minor groove width potentials, melting temperature in all possible combination, using scanning windows of variable size (see Fig. 3). For each function used, a cut-off value has to be set. The program returns a hit every time the computed score of a given region is above the set cut-off value for all of the chosen criteria. Two data output modes are available to handle the hits, the first (called “profile-like") simply returns all hit positions on the query sequence and their corresponding values for the different criteria chosen. The second mode (called “contiguous hits ”) returns only the positions of several contiguous hits and their corresponding sequence.
- the minimum number of contiguous hits is another cut-off value that can be set, again with a tunable window size.
- This second mode is the default mode of SMAR Scan®. Indeed, from a semantic point of view, a hit is considered as a core-unwinding element (CUE), and a cluster of CUEs accompanied by clusters of binding sites for relevant proteins is considered as a MAR. Thus, SMAR Scan® considers only several contiguous hits as a potential MAR.
- CUE core-unwinding element
- the default cut-off values of SMAR Scan® for the bend, the major groove depth and the minor groove width were set at the average of the 75th quantile and the median.
- the default cut-off value should be set at the 75th quantile.
- the minimum length for the "contiguous-hits" mode should be set to 300 because it is assumed to be the minimum length of a MAR (see Fig. 8 and 9).
- one skilled in the art would be able to determine the cut-off values for the above-mentioned criteria for a given organism with minimal experimentation.
- DNA bending values are comprised between 3 to 5 ° (radial degree). Most preferably they are situated between 3.8 to 4.4 °, corresponding to the smallest peak of Fig. l
- the major groove depth values are comprised between 8.9 to 9.3 A (Angstrom) and minor groove width values between 5.2 to 5.8 A.
- the major groove depth values are comprised between 9.0 to 9.2 A and minor groove width values between 5.4 to 5.7 A.
- the melting temperature is comprised between 55 to 75 ° C (Celsius degree). Most preferably, the melting temperature is comprised between 55 to 62 ° C.
- the DNA binding protein of which values can be computed by the method is usually a transcription factor preferably a polyQpolyP domain or a transcription factor selected from the group comprising SATB1 , NMP4, MEF2, S8, DLX1, FREAC7, BRN2, GATA 1/3, TATA, Bright, MSX, AP1 , C/EBP, CREBP1 , FOX, Freac7, HFH1 , HNF3alpha, Nkx25, POU3F2, Pirl , TTF1 , XFD1 , AR, C/EBPgamma, Cdc5, FOXD3, HFH3, HNF3 beta, MRF2, Oct1 , POU6F1 , SRF, V$MTATA_B, XFD2, Bach2, CDP CR3, Cdx2, FOXJ2, HFL, HP1 , Myc, PBX, Pax3, TEF, VBP, XFD3, Brn2, COMP1 , Evil, FOXP3, GATA4, HFN
- the above-mentioned method further comprises at least one filter predicting DNA binding sites for DNA transcription factors in order to reduce the computation.
- the principle of this method combines SMAR Scan® to compute the structural features as described above and a filter, such as for example, the pfsearch, (from the pftools package as described in Bucher P, Karplus K, Moeri N, and Hofmann K, "A flexible search technique based on generalized profiles", Computers and Chemistry , 20:324, 1996) to predict the binding of some transcription factors.
- a filter such as for example, the pfsearch, (from the pftools package as described in Bucher P, Karplus K, Moeri N, and Hofmann K, "A flexible search technique based on generalized profiles", Computers and Chemistry , 20:324, 1996) to predict the binding of some transcription factors.
- filters comprise, but are not limited to, pfsearch, Matlnspector, RMatch Professional and TRANSFAC Professional
- This combined method uses the structural features of SMAR Scan® and the predicted binding of specific transcription factors of the filter that can be applied sequentially in any order to select MARs, therefore, depending on the filter is applied at the beginning or at the end of the method.
- the first level selects sequences out of the primary input sequence and the second level, consisting in the filter, may be used to restrain among the selected sequences those which satisfy the criteria used by the filter.
- the filter detects clusters of DNA binding sites using profiles or weightmatrices from, for example, Matlnspector (Quandt K, Freeh K, Karas H, Wingender E, Werner T, "Matlnd and Matlnspector New fast and versatile tools for detection of consensus matches in nucleotide sequence data", Nucleic Acids Research , 23, 48784884, 1995.).
- the filter can also detect densities of clusters of DNA binding sites.
- the combined method is actually a "wrapper” written in Perl for SMAR Scan® and, in case the pfsearch is used as a filter, from the pftools.
- the combined method performs a twolevel processing using at each level one of these tools (SMAR Scan® or filter) as a potential "filter", each filter being optional and possible to be used to compute the predicted features without doing any filtering.
- SMAR Scan® is used in the first level to filter subsequences, it has to be used with the "all the contiguous hits" mode in order to return sequences.
- pfsearch is used in the first level as first filter, it has to be used with only one profile and a distance in nucleotide needs to be provided. This distance is used to group together pfsearch hits that are located at a distance inferior to the distance provided in order to return sequences; The combined method launches pfsearch, parses its output and returns sequences corresponding to pfsearch hits that are grouped together according to the distance provided. Then whatever the tool used in the first level, the length of the subsequences thus selected can be systematically extended at both ends according to a parameter called "hits extension".
- the second and optional level can be used to filter out sequences (already filtered sequences or unfiltered input sequences) or to get the results of SMAR Scan® and/or pfsearch without doing any filtering on these sequences. If the second level of combined method is used to filter, for each criteria considered cutoff values (hit per nucleotide)need to be provided to filter out those sequences (see Fig. 20).
- Another concern of the present invention is also to provide a method for identifying a MAR sequence comprising at least one filter detecting clusters of DNA binding sites using profiles or weightmatrices.
- this method comprises two levels of filters and in this case, SMAR Scan® is totally absent from said method.
- the two levels consist in pfsearch.
- Also embraced by the present invention is a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter.
- all of the "super" MARs detected with the combined method contain at least 10% of dinucleotide TA on a stretch of 100 contiguous base pairs.
- these sequences contain at least 33% of dinucleotide TA on a stretch of 100 contiguous base pairs.
- these same sequences further contain at least 12% of dinucleotide AT on a stretch of 100 contiguous base pairs. Preferably, they contain at least 33% of dinucleotide AT on a stretch of 100 contiguous base pairs.
- An other aspect of the invention is to provide a purified and isolated MAR DNA sequence of any of the preceding described MARs, comprising a sequence selected from the sequences SEQ ID Nos 1 to 27, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- said purified and isolated MAR DNA sequence comprises a sequence selected from the sequences SEQ ID Nos 24 to 27, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- sequences 24 to 27 correspond to those detected by the combined method and show a higher protein production increasing activity over sequences 1 to 23.
- the present invention also encompasses the use of a purified and isolated DNA sequence comprising a first isolated matrix attachment region (MAR) nucleotide sequence which is a MAR nucleotide sequence selected from the group comprising - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants or a MAR nucleotide sequence of a cLysMAR element and/or fragment, a sequence complementary thereof, a part thereof sharing at least
- Said purified and isolated DNA sequence usually further comprises one or more regulatory sequences, as known in the art e.g. a promoter and/or an enhancer, polyadenylation sites and splice junctions usually employed for the expression of the protein or may optionally encode a selectable marker.
- a promoter and/or an enhancer e.g. a promoter and/or an enhancer, polyadenylation sites and splice junctions usually employed for the expression of the protein or may optionally encode a selectable marker.
- a promoter and/or an enhancer e.g. a promoter and/or an enhancer, polyadenylation sites and splice junctions usually employed for the expression of the protein or may optionally encode a selectable marker.
- a promoter which is operably linked to a gene of interest.
- DNA sequences of this invention can be isolated according to standard PCR protocols and methods well known in the art.
- Promoters which can be used provided that such promoters are compatible with the host cell are, for example, promoters obtained from the genomes of viruses such as polyoma virus, adenovirus (such as Adenovirus 2), papilloma virus (such as bovine papilloma virus), avian sarcoma virus, cytomegalovirus (such as murine or human cytomegalovirus immediate early promoter), a retrovirus, hepatitis-B virus, and Simian Virus 40 (such as SV 40 early and late promoters) or promoters obtained from heterologous mammalian promoters, such as the actin promoter or an immunoglobulin promoter or heat shock promoters.
- viruses such as polyoma virus, adenovirus (such as Adenovirus 2), papilloma virus (such as bovine papilloma virus), avian sarcoma virus, cytomegalovirus (such as murine or human cytomegal
- the purified and isolated DNA sequence might further comprise regulatory sequences which are capable of directing expression of the nucleic acid preferentially in a particular cell type (e. g., tissue-specific regulatory elements are used to express the nucleic acid).
- tissue-specific regulatory elements are known in the art.
- suitable tissue-specific promoters include the albumin promoter (liver- specific; Pinkert,et al., 1987. Genes Dev.1 : 268-277), lymphoid-specific promoters (Calame and Eaton, 1988. Adv. Immunol. 43: 235-275), in particular promoters of T cell receptors (Winoto and Baltimore, 1989. EMBOJ.
- promoters are also encompassed. Examples of such promoters include, e.g., the murine hox promoters (Kessel and Gruss, 1990. Science 249: 374-379) and thea-fetoprotein promoter (Campes and Tilghman, 1989. Genes Dev. 3: 537-546).
- Regulatable gene expression promoters are well known in the art, and include, by way of non-limiting example, any promoter that modulates expression of a gene encoding a desired protein by binding an exogenous molecule, such as the CRE/LOX system, the TET system, the doxycycline system, the NFkappaB/UV light system, the Leu3p/isopropylmalate system, and theGLVPc/GAL4 system (See e. g., Sauer, 1998, Methods 14 (4): 381-92 ; Lewandoski, 2001 , Nat. Rev. Genet 2 (10): 743-55; Legrand- Poels et al., 1998, J. Photochem. Photobiol. B. 45: 18; Guo et al., 1996, FEBS Lett. 390 (2): 191-5; Wang et al., PNAS USA, 1999,96 (15): 84838).
- an exogenous molecule such as the CRE/LOX system
- Enhancers can be optionally included in the purified DNA sequence of the invention then belonging to the regulatory sequence, e.g. the promoter.
- the "gene of interest” or “transgene” preferably encodes a protein (structural or regulatory protein).
- protein refers generally to peptides and polypeptides having more than about ten amino acids.
- the proteins may be “homologous” to the host (i.e., endogenous to the host cell being utilized), or
- heterologous i.e., foreign to the host cell being utilized
- the protein may be produced as an insoluble aggregate or as a soluble protein in the periplasmic space or cytoplasm of the cell, or in the extracellular medium.
- proteins include hormones such as growth hormone or erythropoietin (EPO), growth factors such as epidermal growth factor, analgesic substances like enkephalin, enzymes like chymotrypsin, receptors to hormones or growth factors, antibodies and include as well proteins usually used as a visualizing marker e.g. green fluorescent protein.
- the purified DNA sequence further comprises at least a second isolated matrix attachment region (MAR) nucleotide sequence selected from the group comprising - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- the isolated matrix attachment region (MAR) nucleotide sequence might be identical or different. Alternatively, a first and a second identical MAR nucleotide sequence are used.
- the MAR nucleotide sequences are located at both the 5' and the 3' ends of the sequence containing the promoter and the gene of interest.
- the invention also envisions the fact that said first and or at least second MAR nucleotide sequences are located on a sequence distinct from the one containing the promoter and the gene of interest.
- Embraced by the scope of the present invention is also the purified and isolated DNA sequence comprising a first isolated matrix attachment region (MAR) nucleotide sequence which is a MAR nucleotide sequence selected from the group comprising - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants that can be used for increasing protein production activity in a eukaryotic host cell by introducing the purified and isolated DNA sequence into a eukaryotic
- Usually applied methods for introducing DNA into eukaryotic host cells applied are e.g. direct introduction of cloned DNA by microinjection or microparticle bombardment; electrotransfer ;use of viral vectors; encapsulation within a carrier system; and use of transfecting reagents such as calcium phosphate, diethylaminoethyl (DEAE) -dextran or commercial transfection systems like the Lipofect-AMINE 2000 (Invitrogen).
- the transfection method used to introduce the purified DNA sequence into a eukaryotic host cell is the method for transfecting a eukaryotic cell as described below.
- the purified and isolated DNA sequence can be used in the form of a circular vector.
- the purified and isolated DNA sequence is used in the form of a linear DNA sequence as vector.
- plasmid and “vector” are used interchangeably, as the plasmid is the most commonly used vector form.
- the invention is intended to include such other forms of expression vectors, including, but not limited to, viral vectors (e. g., replication defective refroviruses, adenoviruses and adeno-associated viruses), which serve equivalent functions.
- the present invention further encompasses a method for transfecting a eukaryotic host cell, said method comprising a) introducing into said eukaryotic host cell at least one purified DNA sequence comprising at least one DNA sequence of interest and/or at least one purified and isolated DNA sequence comprising a MAR nucleotide sequence or other chromatin modifying elements, b) subjecting within a defined time said transfected eukaryotic host cell to at least one additional transfection step with at least one purified DNA sequence comprising at least one DNA sequence of interest and/or with at least one purified and isolated DNA sequence comprising a MAR nucleotide sequence or other chromatin modifying elements c) selecting said transfected eukaryotic host cell.
- step b Preferably at least two up to four transfecting steps are applied in step b).
- a gene that encodes a selectable marker (e. g., resistance to antibiotics) is generally introduced into the host cells along with the gene of interest.
- the gene that encodes a selectable marker might be located on the purified DNA sequence comprising at least one DNA sequence of interest and/or at least one purified and isolated DNA sequence consisting of a MAR nucleotide sequence or other chromatin modifying elements or might optionally be co-introduced in separate form e.g. on a plasmid.
- selectable markers include those that confer resistance to drugs, such as G418, hygromycin and methotrexate. The amount of the drug can be adapted as desired in order to increase productivity
- one or more selectable markers are used.
- the selectable markers used in each distinct transfection steps are different. This allows selecting the transformed cells that are "multi-transformed" by using for example two different antibiotic selections.
- Any eukaryotic host cell capable of protein production and lacking a cell wall can be used in the methods of the invention.
- useful mammalian host cell lines include human cells such as human embryonic kidney line (293 or 293 cells subcloned for growth in suspension culture, Graham et al., J. Gen Virol 36, 59 (1977)), human cervical carcinoma cells (HELA, ATCC CCL 2), human lung cells (W138, ATCC CCL 75), human liver cells (Hep G2, HB 8065); rodent cells such as baby hamster kidney cells (BHK, ATCC CCL 10), Chinese hamster ovary cells/-DHFR (CHO, Urlaub and Chasin, Proc. Natl. Acad. Sci.
- human embryonic kidney line (293 or 293 cells subcloned for growth in suspension culture, Graham et al., J. Gen Virol 36, 59 (1977)
- human cervical carcinoma cells HELA, ATCC CCL 2
- human lung cells W138, ATCC CCL 75
- mice sertoli cells TM4, Mather, Biol. Reprod 23, 243-251 (1980)
- mouse mammary tumor MMT 060562, ATCC CCL51
- cells from other mammals such as monkey kidney CV1 line transformed by SV4O (COS-7, ATCC CRL 1651); monkey kidney cells (CV1 ATCC CCL 70); African green monkey kidney cells (VERO-76, ATCC CRL-1587); canine kidney cells (MDCK, ATCC CCL 34); buffalo rat liver cells (BRL 3A, ATCC CRL 1442); myeloma (e.g. NS0) /hybridoma cells.
- the selected transfected eukaryotic host cells are high protein producer cells with a production rate of at least 10 pg per cell per day.
- Most preferred for uses herein are mammalian cells, more preferred are CHO cells.
- the DNA sequence of interest of the purified and isolated DNA sequence is usually a gene of interest preferably encoding a protein operably linked to a promoter as described above.
- the purified and isolated DNA sequence comprising at least one DNA sequence of interest might comprise additionally to the DNA sequence of interest MAR nucleotide sequence or other chromatin modifying elements.
- Purified and isolated DNA sequence comprising a MAR nucleotide sequence are for example selected from the group comprising the sequences SEQ ID Nos 1 to 27 and/or particular elements of the cLysMAR e.g. the B, K and F regions as well as fragment and elements and combinations thereof as described above.
- Other chromatin modifying elements are for example boundary elements (BEs), locus control regions (LCRs), and universal chromatin opening elements (UCOEs) (see Zahn-Zabal et al. already cited).
- An example of multiple transfections of host cells is shown in Example 12 (Table 3).
- the first transfecting step is carried out with the gene of interest (SV40EGFP) alone, with a MAR nucleotide sequence (MAR) alone or with the gene of interest and a MAR nucleotide sequence (MAR-SV40EGFP).
- the second transfecting step is carried out with the gene of interest (SV40EGFP) alone, with a MAR nucleotide sequence (MAR) alone or with the gene of interest and a MAR nucleotide sequence (MAR-SV40EGFP), in all possible combinations resulting from the first transfecting step.
- the eukaryotic host cell is transfected by: a) introducing a purified DNA sequence comprising one DNA sequence of interest and additionally a MAR nucleotide sequence, b) subjecting within a defined time said transfected eukaryotic host cell to at least one additional transfection step with the same purified DNA sequence comprising one DNA sequence of interest and additionally a MAR nucleotide sequence of step a).
- the MAR nucleotide sequence of the of the purified and isolated DNA sequence is selected form the group comprising - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- said purified DNA sequence comprising at least one DNA sequence of interest can be introduced in form of multiple unlinked plasmids, comprising a gene of interest operably linked to a promoter, a selectable marker gene, and/or protein production increasing elements such as MAR sequences.
- the ratio of the first and subsequent DNA sequences may be adapted as required for the use of specific cell types, and is routine experimentation to one ordinary skilled in the art.
- the defined time for additional transformations of the primary transformed cells is tightly dependent on the cell cycle and on its duration. Usually the defined time corresponds to intervals related to the cell division cycle.
- the defined time is the moment the host cell just has entered into the same phase of a second or a further cell division cycle, preferably the second cycle.
- This time is usually situated between 6h and 48 h, preferably between 20h and 24h after the previous transfecting event.
- Also encompassed by the present invention is a method for transfecting a eukaryotic host cell, said method comprising co-transfecting into said eukaryotic host cell at least one first purified and isolated DNA sequence comprising at least one DNA sequence of interest, and a second purified DNA comprising at least one MAR nucleotide selected from the group comprising: - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- a process for the production of a protein wherein a eukaryotic host cell is transfected according to the transfection methods as defined in the present invention and is cultured in a culture medium under conditions suitable for expression of the protein. Said protein is finally recovered according to any recovering process known to the skilled in the art.
- the eukaryotic host cell transfected with the transfection method of the present invention is used in a process for the production of a protein by culturing said cell under conditions suitable for expression of said protein and recovering said protein.
- Suitable culture conditions are those conventionally used for in vitro cultivation of eukaryotic cells as described e.g. in WO 96/39488.
- the protein can be isolated from the cell culture by conventional separation techniques such as e.g. fractionation on immunoaffinity or ion-exchange columns; precipitation; reverse phase HPLC; chromatography; chromatofocusing; SDS-PAGE; gel filtration.
- proteins that are produced according to this invention can be tested for functionality by a variety of methods. For example, the presence of antigenic epitopes and ability of the proteins to bind ligands can be determined by Western blot assays, fluorescence cell sorting assays, immunoprecipitation, immunochemical assays and/or competitive binding assays, as well as any other assay which measures specific binding activity.
- proteins of this invention can be used in a number of practical applications including, but not limited to:
- Antigen production for generation of antibodies for immuno-histochemical mapping including mapping of orphan receptors and ion channels.
- the eukaryotic host cell is a mammalian host cell line.
- a mammalian host cell line include human cells such as human embryonic kidney line (293 or 293 cells subcloned for growth in suspension culture, Graham et al., J.
- human cervical carcinoma cells HELA, ATCC CCL 2
- human lung cells W138, ATCC CCL 75
- human liver cells Hep G2, HB 8065
- rodent cells such as baby hamster kidney cells (BHK, ATCC CCL 10), Chinese hamster ovary cells/-DHFR (CHO, Urlaub and Chasin, Proc. Natl. Acad. Sci.
- mice sertoli cells TM4, Mather, Biol: Reprod 23, 243-251 (1980)
- mouse mammary tumor MMT 060562, ATCC CCL51
- cells from other mammals such as monkey kidney CV1 line transformed by SV4O (COS-7, ATCC CRL 1651 ); monkey kidney cells (CV1 ATCC CCL 70); African green monkey kidney cells (VERO-76, ATCC CRL- 1587); canine kidney cells (MDCK, ATCC CCL 34); buffalo rat liver cells (BRL 3A, ATCC CRL 1442); myeloma (e.g. NS0) /hybridoma cells. Most preferred for uses herein are CHO cells.
- the present invention also provides for a cell transfection mixture or Kit comprising at least one purified and isolated DNA sequence according to the invention.
- the invention further comprises a transgenic organism wherein at least some of its cells have stably incorporated at least one DNA sequence of - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- transgenic organisms wherein its genome has stably incorporated at least one DNA sequence of - a purified and isolated DNA sequence having protein production increasing activity, - a purified and isolated MAR DNA sequence identifiable according to the method for identifying a MAR sequence using the described bioinformatic tool, the combined method or the method comprising at least one filter, - the sequences SEQ ID Nos 1 to 27, - a purified and isolated cLysMAR element and/or fragment, - a synthetic MAR sequence comprising natural MAR element and/or fragments assembled between linker sequences, a sequence complementary thereof, a part thereof sharing at least 70% nucleotides in length, a molecular chimera thereof, a combination thereof and variants.
- Transgenic eukaryotic organisms which can be useful for the present invention are for example selected form the group comprising mammals (mouse, human, monkey etc) and in particular laboratory animals such as rodents in general, insects (drosophila, etc), fishes (zebra fish, etc.), amphibians (frogs, newt, etc..) and other simpler organisms such as c. elegans, yeast, etc....
- Yet another object of the present invention is to provide a computer readable medium comprising computer-executable instructions for performing the method for identifying a MAR sequence as described in the present invention.
- SMAR Scan® A first rough evaluation of SMAR Scan® was done by analyzing experimentally defined human MARs and non-MAR sequences.
- MAR sequences the previous results from the analysis of human MARs from SMARt Db were used to plot a density histogram for each criterion as shown in Fig. 1.
- non-MAR sequences were also analyzed and plotted.
- non-MAR sequences all Ref-Seq-contigs from the chromosome 22 were used, considering that this latter was big enough to contain a negligible part of MAR sequences regarding the part of non-MAR sequences.
- the density distributions shown in Fig. 1 are all skewed with a long tail. For the highest bend, the highest major groove depth and the highest minor groove width, the distributions are right skewed. For the lowest melting temperature, the distributions are left-skewed which is natural given the inverse correspondence of this criterion regarding the three others.
- the MAR sequences biphasic distributions with a second weak peak, are actually apparent. And between MAR and non-MAR sequences distributions, a clear shift is also visible in each plot.
- MARs used to insulate transgene from position effects, such as the interferon locus MAR, the beta-globin locus MAR (Ramezani A, Ha iey TS, Hawley RG, "Performance- and safety-enhanced lentiviral vectors containing the human interferon-beta scaffold attachment region and the chicken beta-globin insulator", Blood, 101:4717-4724, 2003), or the apolipoprotein MAR (Namciu, S, Blochinger KB, Fournier REK, "Human matrix attachment regions in-sulate transgene expression from chromosomal position effects in Drosophila melanogaster", Mol. Cell.
- MAR sequences were also used to determine the association between the four theoretical structural properties computed and the AT- content.
- Fig. 2 represents the scatterplot and the corresponding correlation coefficient r for every pair of criteria.
- Example 2 Distribution plots of MAR sequences by organism
- MAR sequences from SMARt DB of other organisms were also retrieved and analyzed similarly as explained previously.
- the MAR sequences density distributions for the mouse, the chicken, the sorghum bicolor and the human are plotted jointly in Fig. 3.
- SMAR Scan® predicted a total of 803 MARs, their average length being 446 bp, which means an average of one MAR predicted per 42 777 bp.
- the total length of the predicted MARs corresponds to 1 % of the chromosome 22 length.
- the AT-content of the predicted regions ranged from 65,1% to 93.3%; the average AT-content of all these regions being 73.5%.
- predicted MARs were AT-rich, whereas chromosome 22 is not AT-rich (52.1% AT).
- SMARTest was also used to analyze the whole chromosome 22 and obtained 1387 MAR candidates, their average length being 494 bp representing an average of one MAR predicted per 24 765 bp.
- the total length of the predicted MARs corresponds to 2% of the chromosome 22.
- 154 predicted MARs are found by both programs, which represents respectively 19% and 11 % of SMAR Scan® and SMARTest predicted MARs.
- SMAR Scan® analyses were performed on randomly shuffled sequences of the chromosome 22 (Fig. 4).
- Shuffled sequences were generated using 4 different methods: by a segmentation of the chromosome 22 into no'noverlapping windows of 10 bp and by separately shuffling the nucleotides in each window; by "scrambling” which means a permutation of all nucleotides of the chromosome; by “rubbling” which means a segmentation of the chro- mosome in fragments of 10 bp and a random assembling of these fragments and finally by order 1 Markov chains, the different states being the all the different DNA dinucleotides and the transition probabilities between these states being based on the chromosome 22 scan.
- Example 4 Analvsis of known matrix attachment regions in the Interferon locus with SMAR Scan®
- SMAR Scan® The accuracy of SMAR Scan® was evaluated using six genomic sequences for which experimentally determined MARs have been mapped. In order to perform a comparison with other predictive tools, the sequences analyzed are the same with the sequences previously used to compare MAR-Finder and SMARTest. These genomic sequences are three plant and three human sequences (Table 1) totalizing 310 151 bp and 37 experimentally defined MARs. The results for SMARTest and MAR-Finder in Table 1 come from a previous comparison (Frisch M, Freeh K, Klingenhoff A, Cartharius K, Liebich I and Werner T, In silico pre-diction of scaffold/matrix attachment regions in large genomic sequences, Genome Research, 12:349-354, 2001.).
- MAR-Finder has been used with the default parameters excepted for the threshold that has been set to 0.4 and for the analysis of the protamine locus, the AT-richness rule has been excluded (to detect the non AT-rich MARs as was done for the protamine locus).
- SMARTest predicted 28 regions as MARs 19 (true positives) of these correlate with experimentally defined MARs (specificity: 68%) whereas 9 (32%) are located in non- MARs (false positives).
- the 19 true positives correspond actually to 14 different experimentally defined MARs (sensitivity: 38%).
- MARFinder predicted 25 regions as MARs, 20 (specificity: 80%) of these correlate with experimentally defined MARs corresponding to 12 different experimentally defined MARs (sensitivity: 32%).
- SMAR Scan® predicted 22 regions, 17 being true positives (specificity: 77%) matching 14 different experimentally defined MARs (sensitivity: 38%).
- the same analysis has been applied to human chromosomes 1 and 2 and lead to the determination of 23 MARs sequences (SEQ ID N° 1 to 23). These sequences are listed in Annex 1 in ST25 format.
- Example 6 Analyses of the whole genome using the combined method (SMAR Scan®-pfsearch)
- This table shows that there are very various gene densities per S/MAR predicted for the different chromosomes (standard deviation represents more than 50% of the mean of the density of genes per S/MAR predicted and the fold difference between the higher and the lower density of genes per S/MAR is 6,5).
- Table 2 also shows that the kb per S/MAR varies less that the density of genes per S/MAR (standard deviation represents 25% of the mean of kb per S/MAR and the fold difference between the higher and the lower kb per S/MAR is 3.2).
- Table 2 Number of S/MARs predicted per chromosome. The number of genes per chromosome corresponds to the NCBI human genome statistics (Build 34 Version 3) (National Center for Biotechnology Information, The NCBI handbook [Internet].
- Cdc5 cell division control protein 5
- Nkx3A homeodomain protein regulated by androgen
- POU1 F1 pituitaryspecific positive transcription factor 1
- Table 3 is a summary of all transcription factors binding prediction (totalizing 20 hits or more) on the 1757 sequences analyzed.
- 6.3 Bioinformatics analysis of predicted "super" MARs for dinucleotide frequencies
- Various computer analysis were performed in order to easily identify "super" S/MAR sequences using an explicit criterion that could be identified without computing.
- a di-nucleotide analysis was performed on the 1757 superMARs, computing each of the 16 possible dinucleotide percentage for each sequence considering both strands in the 5' > 3' direction.
- AT and TA represent respectively at least 18,5 % and 28.6 % of the dinucleotide content of the predicted S/MAR sequences, whereas the minimum percentages for the same dinucleotides in nonS/MAR sequences are respectively 0.3 % and 0%.
- the maximum CC and GG content in S/MAR sequences is 4.2 %, whereas in nonS/MAR sequences the percentages for these two dinucleotides can amount up to 20.8 %.
- SMAR Scan® has been tuned for human sequences and consequently yields little "super"MARs with mouse genomic sequences, its default cutoff values were slightly relaxed for the minimum size of contiguous hits to be considered as S/MAR . , (using 200 bp instead of 300 bp). Analysis by SMAR Scan® of these mouse sequences predicted several S/MARs having high values for the different computed structural features. This finding suggests that the human MAR elements are conserved across species.
- Example 7 Dissection of the chicken Ivsozvme gene 5'- MAR The 3000 base pair 5'-MAR was dissected into smaller fragments that were monitored for effect on transgene expression in Chinese hamster ovary (CHO) cells.
- PCR-amplified fragments were contiguous and cover the entire MAR sequence when placed end-to-end.
- Four copies of each of these fragments were ligated in a head-to-tail orientation, to obtain a length corresponding to approximately half of that of the natural MAR.
- the tetramers were inserted upstream of the SV40 promoter in pGEGFPControl, a modified version of the pGL3Control vector (Promega).
- the plasmid pGEGFPControl was created by exchanging the luciferase gene of pGL3Control for the EGFP gene from pEGFP-N1 (Clontech).
- the 5'-MAR-fragment-containing plasmids thus created were co-transfected with the resistance plasmid pSVneo in CHO-DG44 cells using LipofectAmine 2000 (Invitrogen) as transfection reagent, as performed previously (Zahn-Zabal, M., et al., "Development of stable cell lines for production or regulated expression using matrix attachment regions" J Biotechnol, 2001. 87(1): p. 29-42.). After selection of the antibiotic (G-418) resistant cells, polyclonal cell populations were analyzed by FACS for EGFP fluorescence.
- Transgene expression was expressed at the percentiie of high expressor cells, defined as the cells which fluorescence levels are at least 4 orders of magnitude higher than the average fluorescence of cells transfected with the pGEGFPControl vector without MAR.
- Fig. 5 shows that multimerized fragments B, K and F enhance transgene expression, despite their shorter size as compared to the original MAR sequence. In contrast, other fragments are poorly active or fully inactive.
- Example 8 Specificity of B, K and F regions in the MAR context
- the 5'-MAR was serially deleted from the 5'-end (Fig.6, upper part) or the 3'-end (Fig.6, lower part), respectively.
- the effect of the truncated elements was monitored in an assay similar to that described in the previous section.
- Figure 6 shows that the loss of ability to stimulate transgene expression in CHO cells was not evenly distributed.
- the 465 bp F fragment was further dissected into smaller sub-fragments of 234, 243, 213 bp and 122, 125 and 121 bp, respectively. Fragments of the former group were octamerized (8 copies) in a head-to-tail orientation, while those of the latter group were similarly hexa-decamerized (16 copies), to maintain a constant length of MAR sequence. These elements were cloned in pGEGFPControl vector and their effects were assayed in CHO cells as described previously. Interestingly, fragment Fill retained most of the activity of the full-length F fragment whereas fragment Fll, which contains the right-hand side part of fragment Fill, lost all the ability to stimulate transgene expression (Fig. 7).
- Fig. 8 A Analysis of the distribution of individual motifs within the lysozyme gene 5'-MAR is shown in Fig. 8 A, along with some additional motifs that we added to the analysis. Most of these motifs were found to be dispersed throughout the MAR element, and not specifically associated with the active portions. For instance, the binding sites of transcription factors and other motifs that have been associated with MARs were not preferentially localized in the active regions. It has also been proposed that active MAR sequences may consist of combination of distinct motifs. Several computer programs (MAR Finder, SMARTest, SIDD duplex stability) have been reported to identify MARs as regions of DNA that associate with the DNA matrix.
- Nucleosome-favouring sequences may be modelled by a collection of DNA features that include moderately repeated sequences and other physico-chemical parameters that may allow the correct phasing and orientation of the DNA over the curved histone . surface. Identification of many of these DNA properties may be computerized, and up to 38 different such properties have been used to predict potential nucleosome positions. Therefore, we set up to determine if specific components of nucleosome prediction programs might correlate with MAR activity, with the objective to construct a tool allowing the identification of novel and possibly more potent MARs from genomic sequences. To determine whether any aspects of DNA primary sequence might distinguish the active B, K and F regions from the surrounding MAR sequence, we analyzed the 5'- MAR with MAR Scan®.
- MAR B, K and F regions coincides with maxima for DNA bending, major groove depth and minor groove width.
- minima of the DNA melting temperature was also noted with minima of the DNA melting temperature, as determined by the GC content.
- mapping over the MAR F fragment indicated that the melting temperature valley and DNA bending summit indeed correspond the FIB sub-fragment that contains the MAR minimal domain (Fig. 9B).
- active MAR portions may correspond to regions predicted as curved DNA regions by this program, and we will refer to these regions as CUE-B, CUE-K and CUE- F in the text below.
- SATB1 special AT-rich binding protein 1
- NMP4 nuclear matrix protein 4
- MEF2 myogenic enhancer factor 2
- Example 11 Construction of artificial MARs by combining defined genetic elements
- the cLysMAR was deleted of all three CUE regions (Fig. 11, middle part), which resulted in the loss of part of its activity when compared to the complete MAR sequence similarly assembled from all of its components as a control (Fig. 11, top part). Consistently, one copy of each CUE alone, or one copy of each of the three CUEs assembled head-to-tail, had little activity in the absence of the flanking sequences.
- the sequences flanking the CUE-F element were amplified by PCR and assembled to bracket the various CUEs, keeping their original orientation and distance, or without a CUE. These engineered ⁇ 1.8 kb MARs were then assayed for their ability to enhance transgene expression as above. All three CUE were active in this context, and therefore there action is not restricted to one given set of flanking sequences. Interestingly, the CUE-K element was even more active than CUE-F when inserted between the CUE-F flanking sequences, and the former composite construct exhibited an activity as high as that observed for the complete natural MAR (4.8 fold activation).
- CUE-K element What distinguishes the CUE-K element from CUE-F and CUE-B is the presence of overlapping binding sites for the MEF-2 and SatB1 proteins, in addition to its CUE feature. Therefore, fusing CUE-B with CUE-F-flanking domain results in a higher density of all three binding sites, which is likely explanation to the increased activity.
- assemblies of CUEs with sequences containing binding sites for proteins such as NMP4, MEF-2, SatB1 , and/or polyPpolyQ proteins constitute potent artificial MAR sequences.
- Plasmid pPAG01 is a 5640 bp pUC19 derivative. It contains a 2960 bp chicken DNA fragment cloned in BamH1 and Xbal restriction sites. The insert comes from the border of the 5'-end of the chicken lyzozyme locus and has a high A/T-content.
- Plasmid pGEGFP (also named pSV40EGFP) control is a derivative of the pGL3- control vector (Promega) in which the luciferase gene sequence has been replaced by the EGFP gene sequence form the pEGFP-N1 vector (Clontech).
- the size of pGEGFP plasmid is 4334bp.
- Plasmid pUbCEGFP control is a derivative of the pGL3 wit an Ubiquitin promoter.
- Plasmid pPAGOIGFP (also named pMAR-SV40EGFP) is a derivative of pGEGFP with the 5'-Lys MAR element cloned in the MCS located just upstream of the SV40 promoter.
- the size of the pPAGOIEGF plasmid is 7285bp.
- Example 13 Effect of the additional transfection of primary transfectant cells on transgene expression
- cells were plated in a 24-well plate, in growth medium at a density of 1.35 x 10 5 cells/well for CHO-DG44 cells. 16 hours post-inoculum, cells were transfected when they reached 30-40% confluence, using Lipofect-AMINE 2000 (hereinafter LF2000), according to the manufacturer's instructions (Invitrogen). Twenty- seven microliters of serum free medium (Opti-MEM; Invitrogen) containing 1.4 ⁇ l of LF2000 were mixed with 27 ⁇ l of Opti-MEM containing 830 ng of linear plasmid DNA.
- Opti-MEM serum free medium
- the antibiotic selection plasmid (pSVneo) amounted to one tenth of the reporter plasmid bearing the GFP transgene.
- the mix was incubated at room temperature for 20 min, to allow the DNA-LF2000 complexes to form.
- the mixture was diluted with 300 ⁇ l of Opti-MEM and poured into previously emptied cell-containing wells. Following 3 hours incubation of the cells with the DNA mix at 37°C in a CO 2 incubator, one ml of DMEM-based medium was added to each well. The cells were further incubated for 24 hours in a CO 2 incubator at 37°C. The cells were then transfected a second time according to the method described above, except that the resistance plasmid carried another resistance gene (pSVpuro).
- Fig.13 shows that the phenotype of the twice-transfected cells (hereafter called secondary transfectants) not only was strongly coloured, such that special bulb and filter were not required to visualize the green color from the GFP protein, but also contained a majority of producing cells (bottom right-hand side FACS histogram) as compared to the parental population (central histogram).
- This level of fluorescence corresponds to specific cellular productivities of at least 10 pg per cell per day. Indeed, cells transfected only one time (primary transfectants) that did not express the marker protein were almost totally absent from the cell population after re-transfection. Bars below 10 1 units of GFP fluorescence amounted 30% in the central histogram and less than 5% in the right histogram. This suggested that additional cells had been transfected and successfully expressed GFP.
- Table 7 Effect of re-transfecting primary transfectants at 24 hours interval on GFP expression. Two independent experiments are shown.
- the resistance plasmid pSVneo was co-transfected with various GFP expression vectors. One day post- transfection, cells were re-transfected with the same plasmids with the difference that the resistance plasmid was changed for pSVpuro. Cells carrying both resistance genes were selected on 500 ⁇ g/ml G-418 and 5 ⁇ g/ml puromycin and the expression of the reporter gene marker was quantified by Fluoroscan. The fold increases correspond to the ratio of fluorescence obtained from two consecutive transfections as compared to the sum of fluorescence obtained from the corresponding independent transfections.
- Plasmid recombination events occur within a 1-h interval after the plasmid DNA has reached the nucleus and the frequency of homologous recombination between co-injected plasmid molecules in cultured mammalian cells has been shown to be extremely high, approaching unity (Folger, K.R., K. Thomas, and M.R. Capecchi, Nonreciprocal exchanges of information between DNA duplexes coinjected into mammalian cell nuclei. Mol Cell Biol, 1985. 5(1): p.
- the order of plasmid transfection is important, and that the first transfection event should contain a MAR element to allow significantly higher levels of transgene expression. If MAR elements favoured the homologous recombination of the plasmids remaining in episomal forms from the first and second transfection procedures, followed by their co- integration at one chromosomal locus, one would expect that the order of plasmid transfection would not affect GFP levels. However, the above findings indicate that it is more favourable to transfect the MAR element in the first rather than in the second transfection event. This suggests the following molecular mechanism: during the first transfection procedure, the MAR elements may concatemerize and integrate, at least in part, in the cellular chromosome.
- This integrated MAR DNA may in turn favour the further integration of more plasmids, during the second transfection procedure, at the same or at a nearby chromosomal locus.
- Example 15 MARs as long term DNA transfer facilitators If integrated MARs mediated a persistent recombination-permissive chromosomal structure, one would expect high levels of expression even if the second transfection was performed long after the first one, at a time when most of the transiently introduced episomal DNA has been eliminated. To address this possibility, the cells from Table 3, selected for antibiotic resistance for three weeks, were transfected again once or twice and selected for the incorporation of additional DNA resistance markers. The tertiary, or the tertiary and quaternary transfection cycles, were performed with combinations of pMAR or pMAR-SV40EGFP, and analyzed for GFP expression as before.
- MARs act as facilitator of DNA integration.
- the pMAR-SV40EGFP/ pMAR-SV40EGFP secondary transfectants were used in a third cycle of transfection at the end of the selection process.
- the tertiary transfection was accomplished with pMAR or pMAR-SV40EGFP, and pTKhygro as selection plasmid, to give tertiary transfectants.
- cells were transfected again with either plasmid and pSVdhfr, resulting in the quaternary transfectants which were selected in growth medium containing 500 ⁇ g/ml G-418 and 5 ⁇ g/ml puromycin, 300 ⁇ g/ml hygromycin B and 5 ⁇ M methotrexate.
- the secondary transfectants initially exhibited a GFP fluorescence of 8300.
- the fold increases correspond to the ratio of fluorescence obtained from two consecutive transfections as compared to the sum of fluorescence obtained from the corresponding independent transfections.
- the fold increases that were judged significantly higher are shown in bold, and correspond to fluorescence values that are 2-fold higher than the addition of those obtained from the independent transfections.
- MAR elements favour secondary integration events in increasing recombination frequency at their site of chromosomal integration by relaxing closed chromatin structure, as they mediate a local increase of histone acetylation (Yasui, D., et al., SATB1 targets chromatin remodelling to regulate genes over long distances. Nature, 2002. 419(6907): p. 641-5.].
- MARs potentially relocate nearby genes to subnuclear locations thought to be enriched in trans-acting factors, including proteins that can participate in recombination events such as topoisomerases. This can result in a locus in which the MAR sequences can bracket the pSV40EGFP repeats, efficiently shielding the transgenes from chromatin-mediated silencing effects.
- Example 16 Use of MARs identified with SMAR Scan® II to increase the expression of a recombinant protein.
- Four MAR elements were randomly selected from the sequences obtained from the analysis of the complete human genome sequence with SMAR Scan® or the combined method. These are termed 1_6, 1 42, 1_68, (where the first number represents the chromosome from which the sequence originates, and the second number is specific to the predicted MAR along this chromosome) and X_S29, a "super" MAR identified on chromosome X.
- MARs were inserted into the pGEGFPControl vector upstream of the SV40 promoter and enhancer driving the expression of the green fluorescent protein and these plasmids were transfected into cultured CHO cells, as described previously (Zahn-Zabal, M., et al., Development of stable cell lines for production or regulated expression using matrix attachment regions. J Biotechnol, 2001. 87(1): p. 29-42). Expression of the transgene was then analyzed in the total population of stably transfected cells using a fluorescent cell sorter (FACS) machine. As can be seen from Fig.
- FACS fluorescent cell sorter
- Example 17 Effect on hematocrit of in vivo expression of mEpo by electrotransfer of Network system with and without Human MAR (1-68).
- the therapeutic gene encodes EPO (erythropoietin), an hormone used for the treatment of anemia.
- the EPO gene is placed under the control of a doxycycline inducible promoter, in a gene switch system described previously called below the Network system (Imhof, M. O., Chatellard, P., and Mermod, N. (2000).
- mice were injected by the Network system expressing EPO without the 1_68 MAR and 16 other mice were injected with the Network system incorporating the MAR in 5' of the promoter/enhancer sequences driving the expression of the activator and EPO genes.
- half of the mice were submitted to doxycycline in drinking water from the beginning of the experiment (day 0 - the day of electrotransfer) and in the other half, doxycycline was put in drinking water starting at day 21.
- Blood samples were collected using heparinated capillaries by retro-orbital punction at different times after the injection of plasmids.
- the MAR likely protects the transgenes from silencing and allows induction of its expression even after prolong period in non-inducing conditions.
- the MAR element is able to increase the expression of the therapeutic gene as detected from its increased physiological effect on the hematocrit.
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