WO1999052563A9 - A method for the targeting of proteins produced by yersinia into the cytosol of eukaryotic cells - Google Patents
A method for the targeting of proteins produced by yersinia into the cytosol of eukaryotic cellsInfo
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- WO1999052563A9 WO1999052563A9 PCT/US1999/008209 US9908209W WO9952563A9 WO 1999052563 A9 WO1999052563 A9 WO 1999052563A9 US 9908209 W US9908209 W US 9908209W WO 9952563 A9 WO9952563 A9 WO 9952563A9
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- cells
- yersinia
- polypeptide
- yope
- protein
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/63—Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
- C12N15/79—Vectors or expression systems specially adapted for eukaryotic hosts
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- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/195—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
- C07K14/24—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Enterobacteriaceae (F), e.g. Citrobacter, Serratia, Proteus, Providencia, Morganella, Yersinia
Definitions
- This invention is directed to a method for targeting proteins produced by Yersinia to the cytosol of eukaryotic cells and targeting signals that can be used in these methods.
- proteins particularly recombinant proteins, produced by bacteria to the cytosol of eukaryotic cells.
- proteins can be targeted for diagnostic or therapeutic purposes.
- proteins that can be targeted are antibodies, toxins, receptor proteins, and polypeptide hormones.
- such a method would not depend on the specific structural features of the proteins to be targeted and could be used with virtually any fusion protein and with a broad range of eukaryotic cells.
- such a method preserves the three-dimensional structure and activity of the translocated proteins and is performed under conditions that do not expose such proteins to denaturing or destabilizing conditions.
- such a method is also suitable for a broad range of applications of the translocated proteins, such as screening.
- Yops were located in either the eukaryotic cytosol, the extra-cellular medium or remained associated with the bacteria. We could not detect an extra-cellular intermediate for those Yops that were localized to the HeLa cytosol. Targeting depended on the binding of SycE chaperone to YopE residues 15-100 in the Yersinia cytoplasm. During infection of HeLa cells, the signal for YopE export in low calcium-induced Yersiniae (codons 1-15) did not lead to secretion into the extracellular medium.
- a method according to the present invention comprises:
- nucleic acid segment encoding a fusion protein
- the fusion protein including: (a) a composite YopE targeting signal; and (b) a polypeptide to be translocated, the nucleic acid segment being expressed in Yersinia cells;
- the Yersinia species is Y. enterocolitica or Y. pseudotuberculosis.
- the Yersinia species employed is Y. enterocolitica.
- the eukaryotic cells can be animal cells, such as mammalian cells, including human cells.
- the eukaryotic cells can be of a cell type selected from the group consisting of fibroblasts, epithelial cells, and leukocytes.
- the eukaryotic cells can be plant cells.
- the polypeptide can be selected from the group consisting of an antibody, an enzyme, a receptor protein, a hormone, and a toxin.
- the polypeptide can further comprise a reporter segment.
- the composite targeting signal comprises the amino acid sequence M-K-I-S-S-F-I-S-T-S-L-P-L-P-A-S-V-S-G-S-S-S-V-G-E-M-S-G-R-S- V-S-Q-Q-K-S-D-Q-Y-A-N-N-L-A-G-R-T-E-S-P-Q-G-S-S-L-A-S-R-I-I-E-R-L-S-M-A- H-S-V-I-G-F-I-Q-R-M-F-S-E-G-S-H-K-P-V-V-T-P-A-L-T-P-A-Q-M-P-S-P-T (SEQ ID NO: 1).
- the first fifteen amino acids of the composite targeting signal can be M-K-I-S-S-F-I-S-T-S-L-P-L-P-A (SEQ ID NO: 1).
- residues 16-100 of the composite targeting signal can be selected from the group consisting of: (1) S-N-S-G-S-S-S-V-G-E-M-S-G-R-S-V-S-Q-Q-K-S-D-Q-Y-A-N-N-L-A-
- sequences that include are modified from residues 16-100 of SEQ ID NO: 1 by one or more of the following conservative amino acid substitutions:
- valine for either isoleucine or leucine
- the first fifteen amino acids of the composite targeting signal are encoded by a mRNA sequence of
- the first fifteen amino acids of the composite targeting signal are encoded by a mRNA sequence that is selected from the group consisting of:
- the first fifteen amino acids of the targeting signal can be encoded by a mRNA including the sequence AAAAUAU that is part of the first loop of SEQ ID NO: 2.
- Another aspect of the present invention is a method for delivering a peptide to the cytosol of a eukaryotic cell comprising the steps of:
- nucleic acid segment encoding a fusion protein
- the fusion protein including: (a) a targeting signal effective for targeting in a Gram-negative bacterium possessing a Type III translocation mechanism homologous or substantially homologous to the translocation mechanism of Yersinia; and (b) a polypeptide to be translocated, the nucleic acid segment being expressed in the cells of the Gram-negative bacterium;
- the targeting signal can include a second portion that is specific for a protein that has substantial homology with the SycE protein of Yersinia at its carboxy-terminal end and has chaperone function.
- Another aspect of the present invention is a method for blocking the introduction of a bacterial protein translocated by a translocation system in a Gram-negative bacterium employing a targeting signal into a eukaryotic cell comprising inhibiting the transcription or translation of mRNA for a protein of the translocation system having protein targeting activity by administering at least one antisense oligonucleotide to inhibit the transcription or translation of the protein having protein targeting activity.
- the Gram-negative bacterium is a Yersinia species and the protein of the translocation system is the Yersinia YopE protein.
- Yet another aspect of the present invention is a method for screening for the activity of a translocated polypeptide in a eukaryotic cell.
- the method comprises: (1) providing a translocated polypeptide in a eukaryotic cell by:
- a nucleic acid segment encoding a fusion protein including: (i) a composite YopE targeting signal; and (ii) a polypeptide to be translocated, the nucleic acid segment being expressed in Yersinia cells;
- the detection of the result of the activity of the polypeptide in the eukaryotic cell can be performed by a method selected from the group consisting of detection of an enzymatic activity, detection of an antibody activity, and detection of a specific binding activity.
- the eukaryotic cells into which the fusion protein including the polypeptide is to be translated can be animal or plant cells. If animal cells, they can be mammalian or non- mammalian cells, including amphibian, fish, reptilian, or avian cells. If they are mammalian cells, they can be human or non-human cells. If they are non-human cells, they can be primate or non-primate cells, including feline, canine, bovine, ovine, equine, murine, or other non-primate cells. The method can be used with a large range of cell types, including fibroblasts, epithelial cells, and leukocytes.
- Another aspect of the present invention is a method for screening for the activity of a translocated polypeptide in a eukaryotic cell. This method comprises:
- the translocation process described in the present application represents a novel site for antibiotic action. Accordingly, a process for blocking the introduction of bacterial proteins into eukaryotic cells is within the scope of the present invention. This process can involve inhibiting the transcription or translation of the mRNA for the YopE protein or an analogous protein with antisense technology.
- Figure 1 shows the localization of Yop proteins during HeLa cell infections of Y. enterocolitica; media (Med.) were decanted from HeLa cells and centrifuged to sediment non-adherent bacteria (P, pellet) and separate them from secreted Yops in the supernatant (S); HeLa cells and attached Yersiniae were extracted with digitonin (Dig.) to specifically solubilize the HeLa plasma membrane and release Yop proteins targeted into the eukaryotic cytosol; unlysed bacteria, eukaryotic membranes and organelles were sedimented by centrifugation (P) and separated from the HeLa cytosol in the supernatant (S); as a control for solubilization of all membranes, infected HeLa cells were extracted with SDS followed by centrifugation; proteins were precipitated with chloroform / methanol, separated on SDS- PAGE, electroblotted and immuno-stained with specific antisera; infections were with either, A.
- FIG. 2 shows the targeting signal of YopE:
- D yopNI mutant VTLI (sycE + , yopN) expressing YopE- NPT translational fusions infected HeLa tissue cultures for 3 hours prior to digitonin fractionation as described in the legend to Fig.
- Figure 3 shows immunofluorescent detection of YopE-NPT fusions by confocal laser microscopy; HeLa cells were infected with Y enterocolitica strains expressing YopE-NPT fusion proteins and targeting was detected by indirect immunofluorescence using anti-NPT and Oregon green-conjugated secondary antibody; the HeLa plasma membrane was stained with Texas red-conjugated wheat germ agglutinin. Panels show infections of Y. enterocolitica W22703 harboring A. pDA36 (YopE-NPT), B. pDA44 (YopE O o-NPT), C pDA45 (YopE 1-50 -NPT), D. pDA46 (YopE 5 -NPT), E.
- A. pDA36 YopE-NPT
- B. pDA44 YopE O o-NPT
- C pDA45 YopE 1-50 -NPT
- D. pDA46
- FIG. 4 shows the substrate requirements for YopE secretion and targeting by the type III machinery; YopE-NPT fusion proteins were expressed in either wild-type Y. enterocolitica W22703 or sycEl mutant strain LC2; targeting of YopE-NPT fusions during the infection of HeLa cells was performed as described in the legend to Fig.
- enterocolitica W22703 (pDA36) as described in the legend to Fig. 1 and processed for transmission electron microscopy; thin sections were incubated with antiNPT and protein A-colloidal gold conjugate (9 nm) followed by staining with uranyl acetate and lead; see Table 1 for quantification of gold particles.
- nucleic Acid Sequence includes both DNA and RNA unless otherwise specified, and, unless otherwise specified, includes both double-stranded and single-stranded nucleic acids. Also included are hybrids such as DNA- RNA hybrids.
- a reference to DNA includes RNA that has either the equivalent base sequence except for the substitution of uracil and RNA for thymine in DNA, or has a complementary base sequence except for the substitution of uracil for thymine, complementarity being determined according to the Watson-Crick base pairing rules.
- Reference to nucleic acid sequences can also include modified bases as long as the modifications do not significantly interfere either with binding of a ligand such as a protein by the nucleic acid or with Watson-Crick base pairing.
- antibody includes both intact antibody molecules of the appropriate specificity, and antibody fragments (including Fab, F(ab'), Fv, and F(ab') 2 ), as well as chemically modified intact antibody molecules and antibody fragments, including hybrid antibodies assembled by in vitro reassociation of subunits. Also included are single-chain antibody molecules generally denoted by the term sFv and humanized antibodies in which some or all of the originally non-human constant regions are replaced with constant regions originally derived from human antibody sequences. Both polyclonal and monoclonal antibodies are included unless otherwise specified. Additionally included are modified antibodies or antibodies conjugated to labels or other molecules that do not block or alter the binding capacity of the antibody.
- the method involves one step translocation of the polypeptide in response to targeting signals provided by the first 100 amino acid residues of the YopE protein of the first 100 amino acid residues of the YopE protein of Yersinia.
- This method requires functional SycE chaperone activity.
- the translocated polypeptide is delivered to the cytosol of the eukaryotic cells.
- the improved way of targeting proteins to the cytosol of eukaryotic cells makes use of targeting mechanisms employed by pathogenic bacteria.
- pathogenic bacteria One such class of pathogenic bacteria is the genus Yersinia. Upon entering their human host, most bacteria are phagocytosed and killed by the cellular immune system. Three pathogenic Yersinia species, Y. pestis, Y. pseudotuberculosis and Y.
- enterocolitica have devised a mechanism that, upon direct contact, kills host cells and allows these microbes to multiply within lymphoid tissues and to establish disease (Straley et al., 1993a; Cornelis & Wolf-Watz, 1997), Contact with eukaryotic cells provides a signal for Yersinia to target cytotoxic proteins, Yops (Yersinia out proteins), into the host cells by a type III mechanism (Rosqvist et al, 1994; Petterson et al, 1996).
- Yop proteins interfere with signal transduction and cytoskeletal rearrangement events, thereby allowing Yersinia to evade the infected host's defense (Bliska et al, 1991 ; Galyov et al., 1993; Straley et al., 1993b).
- type III secretion can also be induced by low calcium concentration and temperature shift to 37°C, which results in the secretion of fourteen different Yop proteins into the surrounding medium (Michiels et al, 1990).
- secretion is defined as type III export of Yops into the extra-cellular medium, whereas targeting refers to the localization of Yops into the eukaryotic cytosol.
- the signal sufficient for the secretion of reporter fusions in low calcium-induced cultures has been mapped to the first fifteen codons of Yops (Michiels and Cornelis, 1991; Sory et al., 1995; Schesser et al., 1996).
- YopE This signal is likely encoded within yop mRNA, because frameshift mutations that completely alter its protein sequence promote secretion of the fused reporter proteins (Anderson and Schneewind, 1997).
- a second independent type III export pathway has been revealed for YopE (Cheng et al., 1997). Mutant YopE with a defective secretion signal can be exported in a manner absolutely dependent on the presence of SycE chaperone.
- SycE is a small homodimeric protein that binds to residues 15- 1 00 of YopE in the Yersinia cytoplasm (Wattiau and Cornelis, 1993; Woestyn et al., 1996) and this interaction is also sufficient to initiate YopE into the secretary pathway (Cheng et al., 1997).
- YopE, YopH and YpkA were found in the cytosol of HeLa cells that had been infected with Y pseudotuberculosis (Rosqvist et al., 1994; Persson et al., 1995; Hakansson et al., 1996b).
- Y. enterocolitica were manipulated to express Yop fusions to Bordetella pertussis adenylate cyclase (Cya) which resulted in an increase of cAMP in the eukaryotic cytosol (Sory and
- Yop targeting was proposed to occur by a two step mechanism (Sory et al., 1995).
- Yops may first be exported across the bacterial envelope via their secretion signal (codons 1-15).
- the translocation domain of YopE, YopH and YopM (residues 15-50, 15-71 15-130 respectively) may then target these polypeptides from the medium or the bacterial surface into the eukaryotic cytosol (Sory et al., 1995; Boland et al., 1996).
- this method comprises:
- nucleic acid segment encoding a fusion protein
- the fusion protein including: (a) the composite YopE targeting signal; and (b) a polypeptide to be translocated, the nucleic acid segment capable of expression in Yersinia cells;
- the Yersinia species is Y. enterocolitica or Y. pseudotuberculosis.
- the Yersinia species employed is Y. enterocolitica.
- the method can also be used with other Gram-negative bacterial cells possessing a homologous or substantially homologous translocation mechanism, one designated as Type III.
- These Gram-negative bacterial cells include Escherichia coli, Salmonella spp., Shigella spp., Pseudomonas spp., and Xanthomonas spp. Therefore, within the scope of the present invention are processes employing these Gram-negative bacteria.
- the method is described herein employing Yersinia, but this is not intended to exclude the use of other appropriate Gram-negative bacteria. In general, this method comprises:
- nucleic acid segment encoding a fusion protein
- the fusion protein including: (a) a targeting signal effective for targeting in a Gram-negative bacterium possessing a Type III translocation mechanism homologous or substantially homologous to the translocation mechanism of Yersinia; and (b) a polypeptide to be translocated, the nucleic acid segment being expressed in the cells of the Gram-negative bacterium;
- the eukaryotic cells into which the fusion protein including the polypeptide is to be translated can be animal or plant cells. If animal cells, they can be mammalian or non- mammalian cells, including amphibian, fish, reptilian, or avian cells. If they are mammalian cells, they can be human or non-human cells. If they are non-human cells, they can be primate or non-primate cells, including feline, canine, bovine, ovine, equine, murine, or other non-primate cells. The method can be used with a large range of cell types, including fibroblasts, epithelial cells, and leukocytes.
- nucleic acid segment encoding the polypeptide to be translocated is DNA.
- nucleic acid segment encoding the polypeptide to be translocated is cloned into the Yersinia.
- other methods involving transient expression are also possible and the method of the present invention is not limited to cloned nucleic acid segments.
- Cloning the nucleic acid segment encoding the fusion protein into the Yersinia is performed by standard methods. In general, such cloning involves: (1) isolation of a nucleic acid segment encoding the polypeptide to be translocated; (2) joining the nucleic acid segment to the composite YopE targeting signal; (3) cloning by insertion into a vector compatible with the bacterium in which expression is to take place; and (4) incorporation of the vector including the new chimeric nucleic acid segment into the bacterium.
- nucleic acid segment encoding the protein to be sorted is DNA; however, the use of RNA in certain cloning steps is within the scope of the present invention.
- cDNA When dealing with genes from eukaryotic organisms, it is preferred to use cDNA, because the natural gene typically contains intervening sequences or introns that are not translated.
- a synthetic gene encoding the protein to be sorted can be constructed by standard solid-phase oligodeoxyribonucleotide synthesis methods, such as the phosphotriester or phosphite triester methods. The sequence of the synthetic gene is determined by the genetic code, by which each naturally occurring amino acid is specified by one or more codons.
- the amino acid sequence can be used to construct a degenerate set of probes according to the known degeneracy of the genetic code.
- General aspects of cloning are described, for example, in J. Sambrook et al., "Molecular Cloning: A Laboratory Manual” (2d ed., Cold Spring Harbor Laboratory Press, Cold Spring Harbor, New York, 1989); in B. Perbal, "A Practical Guide to Molecular Cloning” (2d ed., John Wiley & Sons, New York 1988), in S.L. Berger & A.R. Kimmel, "Guide to Molecular Cloning Techniques" (Methods in Enzymology, vol.
- DNA encoding the protein to be sorted is then joined to the composite YopE targeting signal. This is typically accomplished through ligation, such as using Escherichia coli or bacteriophage T4 ligase. Conditions for the use of these enzymes are well known and are described, for example, in the above general references.
- the ligation is done in such a way so that the protein to be sorted and the sorting signal are joined in a single contiguous reading frame so that a single protein is produced. This may, in some cases, involve addition or deletion of bases of the cloned DNA segment to maintain a single reading frame. This can be done by using standard techniques.
- Cloning is typically performed by inserting the cloned DNA into a vector containing control elements to allow expression of the cloned DNA.
- the vector is then incorporated into the bacterium in which expression is to occur, using standard techniques of transformation or other techniques for introducing nucleic acids into bacteria.
- the control elements can be such elements as promoters or operators. These elements and methods for their use are well known in the art and need not be recited further here.
- the polypeptide to be translocated can be any polypeptide capable of expression in a fusion protein.
- the polypeptide can be an antibody, an enzyme, a receptor protein, a hormone, a toxin, or any other polypeptide having a biological or physiological activity.
- the polypeptide can itself be the result of a previous fusion and thus can carry a "tag" or reporter segment.
- Another aspect of the present invention is a method for screening for the activity of a translocated polypeptide in a eukaryotic cell. This method comprises:
- the detection of the result of an activity of the polypeptide can be the detection of an enzymatic activity, an antibody activity, or a specific binding activity, such as those mediated by hormones, toxins, receptor proteins, or other proteins having biological or physiological activity .
- activity refers to all reactions that depend on the three-dimensional structure of the protein and are specific to proteins with that three-dimensional structure.
- the detection of the activity can be done by methods well known in the art, such as the detection of a product of a reaction catalyzed by the protein if the protein has enzymatic activity, the detection of the detection of a labeled specific binding partner, such as an antibody or a small molecule of the appropriate specificity, specifically binding to the polypeptide, or the detection of an effect caused by the introduction of the polypeptide, such as growth or differentiation of the cell into which the polypeptide has been introduced.
- a labeled specific binding partner such as an antibody or a small molecule of the appropriate specificity, specifically binding to the polypeptide
- an effect caused by the introduction of the polypeptide such as growth or differentiation of the cell into which the polypeptide has been introduced.
- the composite YopE targeting signal comprises two regions, both of which are required to be present.
- the first region is the first 15 amino acids of the signal, which is required for the targeting even though it is not required for YopE-directed secretion. (Cheng et al., 1997).
- this portion of the composite signal may be active at the mRNA level rather than at the protein or polypeptide level, because frameshift mutations that disrupt the sequence of the resulting translated protein can nevertheless be effective in the targeting process.
- the second portion of the targeting signal is residues 15-100 of YopE.
- the sequence of residues 1-100 of YopE is given below:
- the conservative amino acid substitutions can be any of the following: (1) any of isoleucine, leucine, and valine for any other of these amino acids; (2) aspartic acid for glutamic acid and vice versa; (3) glutamine for asparagine and vice versa; and (4) serine for threonine and vice versa.
- Other substitutions can also be considered conservative, depending upon the environment of the particular amino acid. For example, glycine (G) and alanine (A) can frequently be interchangeable, as can be alanine and valine (V).
- Methionine (M) which is relatively hydrophobic, can frequently be interchanged with leucine and isoleucine, and sometimes with valine. Lysine (K) and arginine (R) are frequently interchangeable in locations in which the significant feature of the amino acid residue is its charge and the different pK's of these two amino acid residues or their different sizes are not significant. Still other changes can be considered "conservative" in particular environments.
- an amino acid on the surface of a protein is not involved in a hydrogen bond or salt bridge interaction with another molecule, such as another protein subunit or a ligand bound by the protein
- negatively charged amino acids such as glutamic acid and aspartic acid
- Histidine (H) which is more weakly basic than arginine or lysine, and is partially charged at neutral pH, can sometimes be substituted for these more basic amino acids.
- the amides glutamine (Q) and asparagine (N) can sometimes be substituted for their carboxylic acid homologues, glutamic acid and aspartic acid. Accordingly, processes employing targeting signals that contain conservative amino acid substitutions within residues 15-100 of the composite targeting signal are within the scope of the present invention.
- this first portion of the composite targeting signal is recognized at the mRNA level instead of, or possibly in addition to, the protein or polypeptide level (Anderson & Schneewind, 1997).
- the activity of the first portion of the targeting signal may be reduced or abolished. Therefore, also within the scope of the present invention are processes employing targeting signals whose first portion is encoded by a mRNA including therein SEQ ID NO: 2 or frameshift mutations of SEQ ID NO. 2 with the proviso that the hydrophobicity of the segment of the protein encoded by the mRNA including therein any frameshift mutation of SEQ LD NO: 2 is substantially equivalent to that of the hydrophobicity of the segment of the protein encoded by SEQ ID NO: 2.
- This mRNA has a structure of two stems with loops (Anderson & Schneewind, 1997).
- Mutations that abolish translation may be located either within the first loop or its adjacent base pairs; the remainder of the sequence of the mRNA may be more resistant to the destruction or alteration of the function of the first portion of the signal by mutation. Therefore, also within the scope of the present invention are processes employing targeting signals whose first portion is encoded by a mRNA including the sequence within SEQ ID NO: 2 that is part of the first loop. This segment of mRNA has the sequence AAAAUAU. The first and last residues of this segment are base-paired.
- a process for blocking the introduction of bacterial proteins into eukaryotic cells is within the scope of the present invention.
- This process can involve inhibiting the transcription or translation of the mRNA for the YopE protein or an analogous protein with antisense technology, as described in J.A.H. Murray, ed., "Antisense RNA and DNA” (Wiley-Liss, New York, 1992), incorporated herein by this reference.
- Example 2 The invention is illustrated by the following Example. This Example is for illustrative purposes only and are not to be construed as limiting the scope of the invention in any manner.
- HeLa cells and attached Yersiniae were scraped off the culture flasks, extracted with digitonin and centrifuged to separate the bacteria and other insoluble material from the supernatant, containing eukaryotic cytosol.
- a duplicate sample of infected HeLa culture was treated with sodium dodecyl sulfate (SDS) to solubilize all eukaryotic and bacterial membranes. Protein in all fractions was precipitated with chloroform / methanol and analyzed by immunoblotting.
- SDS sodium dodecyl sulfate
- FPT farnesyl protein-transferase
- YopE, YopH, YopM and YopN were found in the supernatant of digitonin extracted HeLa cells but not in the extracellular medium.
- YopB and YopR were also observed in the pellet fraction of digitonin extracts, whereas YopD was present in all fractions examined.
- YopQ sedimented with the adherent bacteria into the pellet fraction of digitonin extracts.
- YopE, YopH, YopM and YopN were located in the eukaryotic cytosol, whereas other Yops were either secreted (YopB and YopR) or remained associated with the bacteria (YopQ).
- Yop targeting might be accomplished only by Yersinia that have attached to HeLa cells but not by non-adherent bacteria (Rosqvist et al., 1994; Petterson et al., 1996).
- To measure Yersinia adherence to HeLa cells we counted bacteria in the extracellular medium and those present in detergent extracts by dilution and colony formation. Most bacteria (95%) were attached to HeLa cells during tissue culture infection.
- YopH are sufficient to promote the targeting of adenylate cyclase fusions (Sory et al., 1995). However, about half of all adenylate cyclase fusion protein was located in the extracellular medium (Boland et al., 1996). Because this report was in conflict with our measurements of YopE and YopH localization, we examined the targeting of neomycin phosphotransferase (NPT) (Reiss et al., 1984) fusions to YopE with our fractionation assay (Fig. 2A).
- NPT neomycin phosphotransferase
- Hybrid proteins containing either full length YopE or residues 1-100 of YopE fused to NPT were found in the supernatant of digitonin extracted HeLa cells (34 and 8 1 % respectively), indicating that they had been targeted in a manner similar to wild-type YopE (Fig. 2B).
- fusions containing YopE residues 1-50, 1-15 or NPT alone remained in the pellet of digitonin extracts (0% targeting for all three hybrids). None of the hybrid YopE-NPT proteins were secreted into the extracellular medium.
- the defect of the sycEl strain was specific for the targeting of YopE-NPT fusions, since YopM and YopH were still located in the HeLa cytosol.
- the targeting defect of strain LC2 was due to the mutation carried by the SycEl allele, because it could be complemented by a plasmid encoded wild-type allele.
- YopE-NPT fusions in the cytosol of HeLa cells was visualized with anti-NPT staining and immunofluorescence confocal laser microscopy (Fig. 3).
- the HeLa cell plasma membrane was stained with Texas red-labeled wheat germ agglutinin.
- Targeting of YopE-NPT and YopEi.ioo-NPT could be detected as Oregon green-staining of the HeLa cytosol.
- YopE ⁇ - 5 o-NPT, YopEi-is- NPT or NPT alone yielded the same amount of background staining as a control culture infected with Yersiniae that did not express NPT.
- YopE+i-NPT fusion protein is also secreted by wild-type Yersiniae (Cheng et al, 1997). The SycE dependence of YopE-NPT secretion was tested in Y. enterocolitica LC2.
- enterocolitica strain VTLI enterocolitica strain VTLI (yopNI).
- this mutant strain was temperature sensitive for growth and secreted Yops into the culture medium at 37°C even in the presence of calcium.
- Y. enterocolitica VTLI secreted all Yops into the extracellular medium (Fig. IB).
- Some YopE, YopH and YopM could be found in the supernatant of digitonin extracts, suggesting that the yopNI strain may still be able to promote Yop targeting.
- a plasmid encoded wildt.ype.yopN allele restored the fractionation pattern of Yops to that observed for Y. enterocolitica W22703, indicating that the phenotype of strain VTLI was due to the mutation carried by the yopNI allele.
- YopE- ⁇ PT the location of YopE- ⁇ PT fusions was examined during the infection of HeLa cells with Y. enterocolitica VTLI (Fig. 2D).
- YopE- ⁇ PT, YopE 00 - ⁇ PT, YopE 1-5 o-NPT, and YopE ⁇ -1 5 -NPT were secreted into the extra-cellular medium.
- NPT alone as well as YopE-NPT (pDA72) harboring a defective secretion signal, sedimented with the yopNI mutant bacteria.
- the secretion signal located within the first 15 codons of YopE is functional in yopN mutants but not in wildtype Yersiniae.
- YopE-NPT fusions that sedimented after digitonin extraction could be located either in the cytoplasm or on the surface of Yersiniae. If the latter were true, such a result would favor the two step translocation model of Yops, whereas the cytoplasmic location of these NPT fusions would indicate that targeting occurred by a different mechanism.
- the location of YopE-NPT fusions was measured with electron microscopy. When infected with Y.
- YopE-NPT enterocolitica expressing YopE-NPT
- NPT-specific immuno-gold particles were detected in the cytosol of HeLa cells and in the bacterial cytoplasm, but not on the surface o ⁇ Yersiniae (Fig. 5 and Table 1).
- YopE ⁇ . ⁇ 5 -NPT was found in the bacterial cytoplasm but not on cell surfaces or in the HeLa cytosol.
- immuno-gold staining of YopE- NPT was observed only in the bacterial cytoplasm but not in the cytosol of HeLa cells or on cell surfaces. Together these data suggested that YopE-NPT fusions that were not targeted into the HeLa cytosol remained within the bacterial cytoplasm.
- ⁇ opE-NPT fusion proteins were detected with anti-NPT followed by protein A-gold conjugate staining. Gold particles were counted and averaged per bacterium or cm of H HeeLLaa ccyyttooppllaassmm.. DDaattaa wweerree ggaatthheerreedd ffrroomm 2255 bbaaccteria.
- the second mode of type III secretion requires the binding of SycE to residues 15-100 of YopE (Cheng et al., 1997). This interaction is also sufficient for the secretion of reporter fusions in low-calcium induced cells.
- SycE binding to YopE is absolutely necessary for YopE targeting into the HeLa cytosol.
- Forsberg and co-workers have investigated the SycE/YerA requirement with immunofluorescent microscopy and reported a low level targeting of YopE in ayerA mutant of Y. pseudotuberculosis (Frithz-Lindsten et al., 1995). Our experiments compared the digitonin fractionation with immunofluorescent microscopy and we find that the latter is less sensitive.
- YopQ YopK
- Y. pseudotuberculosis Y. pseudotuberculosis during HeLa cell infections
- Adenylate cyclase fusions to YopN did not yield an increase of cAMP during the infection of macrophages by Y. enterocolitica (Boland et al., 1996).
- YopN-NPT fusions did not acquire such digitonin solubility, suggesting that the discrepancies between the two experimental approaches can be explained by the aberrant subcellular location of Yop fusion proteins.
- YopE is targeted directly from the bacterial cytoplasm into the cytosol of HeLa cells. Translocation across three membranes may be achieved by a type III secretion channel spanning the bacterial inner and outer membranes, which may be extended by other, hitherto unknown, proteins into the eukaryotic cytosol.
- YopB and YopD proteins are absolutely required for targeting (Hakansson et al., 1996a), it is believed that these polypeptides might fulfill such a role.
- the substrate requirements for YopE targeting are residues 1-100 bound to SycE chaperone. Because none of the targeted Yops (YopE, YopH, YopM, YopN and YopO) display sequence homology we think it is likely that the Syc proteins play an important role in substrate recognition. For example, a conserved C-terminal sequence element (Wattiau et al. , 1996) or other features of these secretion chaperones could be recognized by the type III machinery. If chaperone delivery to the type III machinery were a universal feature of Yop targeting, one would predict the existence of other Syc proteins (for YopM, YopN and YopO) that have not yet been identified (Wattiau et al. , 1994).
- Yop proteins require the type III machinery for their export from the bacterial cytoplasm (Allaoui et al., 1995).
- One explanation for the different locations of Yop proteins, i.e. the medium, HeLa cytosol or associated with the bacteria, would be that their structural genes are expressed at different times during tissue culture infection.
- Yop proteins that are synthesized once the Yersinia have docked on the surface of HeLa cells might be directed into the eukaryotic cytosol, whereas others, that were expressed prior to attachment, might be secreted.
- An alternative explanation for the different locations of Yop proteins would be that Yersinia switch the mode of substrate recognition for the type III machinery.
- Yops might first be secreted into the medium by an mRNA encoded signal. Later during infection, perhaps after docking of the bacteria on the surface of HeLa cells, type III export may occur only if Yops are properly delivered by their chaperones. It is equally plausible that Yersinia employ both regulatory elements, gene expression and alternate modes of substrate recognition, to position their Yops proteins at different locations relative to the eukaryotic target cell.
- Yersinia strains were grown in Luria broth at 26°C with 150 rpm shaking, diluted 1 :20 into fresh media and incubated for another 2 hours (OD 6 oo 0.4).
- HeLa cells were grown in Dulbecco's minimal eagle medium (DMEM) supplemented with 10% FBS to confluency (2.5 x 10 7 cells per 75 cm 2 flask). Cells were washed twice with 5 ml PBS, incubated in 10 ml DMEM for 30 minutes, infected with Y. enterocolitica [2.5 x 10 8 bacteria, multiplicity of infection (MOI) 10] and incubated for 3 hours at 37°C, 5% CO 2 . Media were collected by decanting and placed on ice.
- DMEM Dulbecco's minimal eagle medium
- HeLa cells attached to the flasks were lysed by the addition of 10 ml PBS containing either 1% purified digitonin or 1% SDS and 10 mM EDTA. Detergent solutions were incubated for 20 min at room temperature with vigorous intermittent vortexing. Samples were sedimented by centrifugation at 20,000 g for 15 minutes. A 6.6 ml portion of supernatant was transferred to a new tube and the remainder discarded. The sediment was suspended in 10 ml of 1% SDS in PBS and a 6.6 ml portion transferred to a new tube.
- Protein was precipitated with methanol / chloroform (Wessel and Flugge, 1984), and suspended in 400 III sample buffer (10% glycerol, 1% SDS, 0.1% bromophenol blue, 5.5 M urea, 2% ⁇ -mercaptoethanol, 36 mM Tris-HCl, pH 6.8). Proteins were separated on SDS-PAGE, electrotransferred onto PVDF membrane, immunoblotted with specific antiserum, and identified as a chemiluminescent signal on X-ray film.
- HeLa cells (2 x 10 5 ) were grown in DMEM on cover slips in a 24 well plate for 48 hours at 37°C, 5% CO 2 . Cells were washed twice with PBS, covered with 1 ml DMEM, and infected with 8 x 10 6 bacteria (MOI of 10) for 3 hours. Samples were first washed with PBS and then fixed with 3.7% formaldehyde in PBS for 20 minutes. The reaction was quenched by washing in PBS and then adding 0.1 M glycine for 5 minutes. HeLa cells were permeabilized with 1% Triton in PBS for 30 minutes.
- Samples were blocked for nonspecific staining with 5% nonfat milk, 0.05% Tween 20 in PBS for 15 minutes followed by incubation with anti-NTT (1 : 100 dilution) for 20 minutes. Samples were washed four times with PBS 0.05% Tween 20 for 5 minutes each and incubated with goat anti-rabbit IgG Oregon 488 green- conjugate as well as wheat germ agglutinin Texas Red-conjugate (Molecular Probes, both diluted 1 :500) for 20 minutes. Samples were washed four times, dried for 1 hour and viewed under a Leica confocal laser microscope.
- HeLa cells were infected with Yersinia and incubated for 3 hours at 37°C, 5% CO 2 as described above. Cells were washed with 10 ml of PBS, scraped off the plate and fixed overnight at 4°C in 2% formaldehyde, 6% sucrose in PBS. Samples were washed twice with PBS and the remaining formaldehyde was quenched with 0.01 M glycine in PBS for 10 minutes. The samples were dehydrated through a graded series of ethanol, placed in resin through a graded series of ethanol-LR White mixtures and baked overnight at 55°C to dry the resin. The embedded cells were cut with an ultra-microtome and thin sections were collected on formvar-coated nickel grids.
- Samples were immuno-stained at room temperature by floating the grids on a series of 50 ⁇ l droplets of different solutions: blocking in 50 mM HEPES, 0.3 M NaCl, 0.05% NaN 3 , 1 % BS A, 0.01 % cold water fish skin gelatin for 30 min, anti-NPT 1 :5 in blocking solution for 1 hour, 7 washes with 50 mM HEPES, 0.3 M NaCl, 0.05% NaN 3 , protein A-colloidal gold conjugate (9 nm particles) 1 :50 in blocking solution for 1 hour, and finally another 7 washes.
- Yops were precipitated from the supernatant of low-calcium induced Y. enterocolitica strain 8081 cultures (Portnoy et al, 1981) with ammonium sulfate (46%>). Precipitated Yops were suspended in 6 M guanidine-HCl, 0.01 M phosphate buffer, 10 mM DTT and separated by reverse phase HPLC on C8 column (Anderson and Schneewind, 1997). YopE, H, M and YopN were purified in this manner. The coding sequences for YopB, D and YopR were PCR amplified with primers specifying abutted BamHl restriction sites for cloning into the pQE vectors (Qiagen).
- Histidine tagged polypeptides were overexpressed in E. coli and purified by affinity chromatography on NI-NTA followed by separation on reverse phase HPLC. Purified polypeptides were injected into rabbits for antibody production, whereas antisera against FPT (Signal Transductions), NPT (5'->3') and TFIID (Oncogen Research) were purchased.
- Plasmids pVL33 and pVL35 were generated by inserting annealed oligonucleotides specifying the codons 1-15 of either cat or lacZ between the Ndel and Kpnl sites of pDA 139. Plasmids were sequenced for confirmation and transformed into Yersinia strains.
- the Y. enterocolitica strains W22703 (Cornelis and Colson, 1975) and LC2 (sycEl) (Cheng et al., 1997) have been described previously.
- the yopNI mutant strain has a stop codon followed by a nucleotide insertion and BamHl site inserted at codon four of the O ?N gene (Forsberg et al., 1991).
- the yopNI mutation was introduced by allele replacement following a standard protocol (Cheng et al, 1997). Procedures to measure Yop secretion by Yersinia strains have been previously reported (Anderson and Schneewind, 1997).
- the surface-located YopN protein is involved in calcium signal transduction in Yersinia pseudotuberculosis. Mol Microbiol 5: 977-986.
- a secreted protein kinase o ⁇ Yersinia pseudotuberculosis is an indispensible virulence determinant . Nature 361: 730-732.
- YopB protein o ⁇ Yersinia pseudotuberculosis is essential for the translocation of Yop effector proteins across the target cell plasma membrane and displays a contact-dependent membrane disrupting activity.
- the present invention provides a widely applicable and efficient method for translocating cloned proteins into eukaryotic cells.
- the method does not depend on particular structural features of the protein to be translocated and thus can be used with virtually any protein to be translocated, as long as a suitable fusion protein can be prepared.
- the method can also be used with a broad range of eukaryotic cells.
- the method is rapid and efficient.
- the method of the present invention also preserves the three-dimensional structure and activity of the translocated proteins and is performed under conditions that do not expose such proteins to denaturing or destabilizing conditions.
- the method is also suited to a broad range of applications, including screening of the proteins that have been translocated.
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US6962696B1 (en) | 1999-10-04 | 2005-11-08 | Vion Pharmaceuticals Inc. | Compositions and methods for tumor-targeted delivery of effector molecules |
US20030194798A1 (en) | 2001-05-24 | 2003-10-16 | Surber Mark W. | Minicell compositions and methods |
US7396822B2 (en) | 2001-05-24 | 2008-07-08 | Vaxiion Therapeutics, Inc. | Immunogenic minicells and methods of use |
WO2003002021A2 (en) | 2001-06-29 | 2003-01-09 | The Regents Of The University Of California | Biodegradable/bioactive nucleus pulposus implant and method for treating degenerated intervertebral discs |
DE10254165A1 (en) | 2002-11-20 | 2004-06-03 | Icon Genetics Ag | Method for controlling a cellular process in a multicellular organism |
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AU2004263896A1 (en) | 2003-08-08 | 2005-02-17 | Genenews Inc. | Osteoarthritis biomarkers and uses thereof |
JP5265923B2 (en) | 2005-02-07 | 2013-08-14 | ジーンニュース インコーポレーテッド | Biomarkers for mild osteoarthritis and uses thereof |
US8092806B2 (en) * | 2005-04-11 | 2012-01-10 | Yeda Research And Development Co. Ltd. | Chimeric proteins, their preparation and pharmaceutical compositions containing them |
WO2007048074A1 (en) | 2005-10-21 | 2007-04-26 | Genenews Inc. | Method and apparatus for correlating levels of biomarker products with disease |
EP2664339A3 (en) * | 2008-03-17 | 2013-12-11 | Universitätsklinikum Münster | YopM as delivery vehicle for cargo molecules and as biological therapeutic for immunomodulation of inflammatory reactions |
US9597379B1 (en) | 2010-02-09 | 2017-03-21 | David Gordon Bermudes | Protease inhibitor combination with therapeutic proteins including antibodies |
US20130273092A1 (en) * | 2010-10-22 | 2013-10-17 | Trudeau Institute | Uses of yersinia yope peptide, gene and subparts thereof as a plague vaccine component and assays for yersinia pestis-specific t cells |
DK2675474T3 (en) | 2011-02-15 | 2019-04-23 | Vaxiion Therapeutics Llc | THERAPEUTIC COMPOSITIONS AND PROCEDURES FOR TARGETED ADMINISTRATION OF BIOACTIVE MOLECULES BY BACK-TERIAL MINICLES BASED ON ANTIBODY AND FC-CONTAINING TAR-GETING MOLECULES |
US11180535B1 (en) | 2016-12-07 | 2021-11-23 | David Gordon Bermudes | Saccharide binding, tumor penetration, and cytotoxic antitumor chimeric peptides from therapeutic bacteria |
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