CA2086342A1

CA2086342A1 - Method of introducing a peptide into a cytosol

Info

Publication number: CA2086342A1
Application number: CA002086342A
Authority: CA
Inventors: Sjur Olsnes
Original assignee: Individual
Current assignee: FORSKNINGSSTIFTELSEN DET NORSKE RADIUMHOSPITAL
Priority date: 1990-06-27
Filing date: 1991-06-26
Publication date: 1991-12-28
Also published as: HU9204125D0; LTIP835A; JPH06503552A; FI925869A0; NO902871D0; NO175188C; WO1992000099A1; NO902871L; EP0542756A1; HUT63061A; NO175188B; FI925869A; AU653158B2; AU8000191A

Abstract

A method of introducing a peptide into the cytosol by linking the peptide to a bacterial or plant toxin, or a mutant thereof. A
method of preparing a vaccine by linking a peptide to a bacterial or plant toxin, or a mutant thereof to translocate the peptide into the cytosol for subsequent presentation at the cell surface by Class I MHC antigens to elicit a Class I restricted immune response and to expand the relevant population of CD8+ T-lymphocytes.
Vaccines produced by said method and the use thereof against viruses, intracellular bacteria and parasites, and against molecules associated with malignancies.

Description

W092/0~99 PCT/~091/000~3 ~ 8~3~2 Method of introducing a peptide into the cytosol Field of the Invention The present invention is direc~ed to a method of in-S troducing a peptide into the cytosol, and more specifically toa novel principle in vaccine production against viruses, intracellular parasites and bacteria and against malignant cells.

o Backqround of the Invention In the protection against pathogenic organisms and in their elimination antigen presentation by major histocompati-bility antigens (MHC) of class I plays an important role.
Cytotoxic T-lymphocytes recognize cells that express foreign 15 or unusual antigens on their surface and destroy the cells, which is important to eliminate an infection. The same mechan-ism is operating in the elimination of malignant cells. Anti-gen presentation by Class I MHC requires that the antigen to be presented is found in the cytosol or in the endoplasmic 20 reticulum (Germain, R.N. Nature 322, 687-689 (1986)). Extern-ally added polypeptides therefore do normally not elicit a class I response. However, if the antigen is artificially introduced into the cytosol, presentation by MHC Class I may occur (Moore, M.W., Carbone, F.R. & Bevan, M.J. Cell 54, 777-zS 785 (1988)). The rommon way today to immunize against suchstructures is to use attenuated live viruses that are able to enter cells and replicate such that the peptides in question are formed in the cells and can be presented at the cell surface. In this way the population of the relevant cytotoxic 30 CD8~ cells is expanded and upon later exposure to the corres-ponding virulant virus strain, the organism has an immune protection. The problems with this approach are partly due to the fact that the attenuated viruses may sometimes revert to virulence and partly to the problems of making attenuated 35 viruses in many cases. Convenient and non-damaging methods to introduce into the cytosol foreign peptides, such as viral antigens, could th~reforP be useful for vaccine purposes to expand the relevant population of CD8~ MHC Class I restricted cytotoxic T-lymphocytes.

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,, : '' ' ' W092/0~99 PCT/NO91/00~93 208~3'1~ 2 The only established examples of external proteins that enter the cytosol are certain bacterial and plant toxins, such as diphtheria toxin, Pseudomonas aeruqinosa exotoxin A, ricin, abrin, viscumin, modeccin, Shigella toxin, cholera toxin, 5 pertussis toxin (Olsnes, S. & Sandvig, K. In: "I~munotoxins"
(A.E. Frankel, ed.), Kluwer Academic Publishers, Boston 19~8, pp. 39-73; Olsnes, S. & Sandvig, K. In "Receptor-mediated endocytosis" (I. Pas-tan & M.C. Willingham, eds.), Plenum Publ.
Corp., 1985, pp. 195-234). Toxins of this group enter the 10 cytosol where they carry out enzymatic reactions that are deleterious to the cell or to the organism. By gene manipu-lations it is possible to form toxin molecules that are of very low toxicity (Barbieri, J.T. & Collier, R.J. Infect.
Immun. 55, 1647-1651 (1987)). If the toxins were able to carry 15 into cells additional peptide material, such non-toxic mutants could be useful for vaccine purposes to carry into the cytosol anti~enic peptides (Cerundolo et al. Nature 345, 449 (1990)) that can be presented by Class I MHC antigens. Such antigenic sequences can be obtained from a number of viruses, bacteria 20 and parasites, and it is also possible to derive such struc-tures from certain malignant cells.

It is an object of the present invention to provide a mechanism of translocating antigenic peptide se~uences to the 25 cytosol in a safe way to expand the population of cytotoxic T-lymphocytes that are able to react with the corresponding antigen and eliminate those cells that are presenting the antigenic peptides. Although the entry mechanism for the different toxins mentioned above is in principle the same, it ~o has been worked out in most detail in the case of diphtheria toxin. This is the toxin we have used in most of our studies in connection with this application.

Summary of the Invention We here demonstrate that an essentially non-toxic mutant of diphtheria ~oxin is able to translocate to the cyto-sol oligopeptides linked to its N-terminal end. The peptides we have studied are sufficiently different in sequence to allow the conclusion that a wide variety of peptides can be . .
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carried into the cells in the same way.
Thus, the present invention relates to a method of introducing a peptide into -the cytosol by linking the peptide to a bacterial or plant toxin, or a mutant ~hereof. Further, 5 the present invention relates to a method of preparing a vaccine by linking a peptide to a bacterial or plant toxin, or a mutant thereof to translocate the peptide into the cytosol for subsequent presentation at the cell surfac:e by Class I MHC
antigens to elicit a Class I restricted immune response and to 10 expand the relevant population o* CD8~ T-lymphocytes. Also, the present invention relates to vaccines which have been produced by the above-mentioned method, as well as the use of such vaccines against viruses, intracellular bacteria and para-sites, and against molecules associated with malignancies.

Fiaure Leaends FIG. 1. N-terminal extensions of diphtheria toxin.
A. The coding region of the diphtheria toxin gene carrying a triple mutation changing Glu14'3 to Ser, and where 20 Gly~ was replaced by initiator Met placed behind a T3 promotor to give pBD-lS (McGill, S., Stenmark, H., Sandvig, K. &
Olsnes, S.: EMBO J. 8, 2843-2848 (1989)). To obtain pB-B3-D1, pBD-1 was cleaved with NcoI, and an oligonucleotide encoding the oligopeptide MGVDEYNEMPMPVN (referred to as B3) was 25 inserted. pGD-2 encodes diphtheria toxin with its natural signal sequence, MSRKLFASILIGALLGIGAPPSAHA (referred to as ss), after an SP6 promotor. The plasmid was obtained by digesting pGD-l (McGill, S., Stenmark, H., Sandvig, K. ~
Olsnes, S.: EMBO J. 8, 2843-2848 (1989)) with HindIII and 30 PstI, removing the overhangs with S1-nuclease and religating to form pGD-2.
B. The genes were transcribed in vitro and the mRNAs obtained were translated in rahbit reticulocyte lysate systems in the presence of [35S]methionine (McGill, S., Stenmark, H., 3S Sandvig, K. & Olsnes, S.: EMBO J. 8, 2843-2848 (1989)). To remove reducing agents and to allow disulfide bridges to be formed, the translation mixture was dialyzed over night against PBS ( O. 14 M NaCl, 10 mM Na-phosphate, pH 7.4), and then for 4 h against Hepes medium (Dulbecco-modified Eagles .~

W092/0~99 PCT/NO91/00093 ~ ' ~ 3 1 2 4 ~
medium wherein the bicarbonate had been replaced by ~O mM
Hepes, pH 7.4). An ali~uot of each sample was analyzed by polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulfate ~SDS-PAGE) under reducing cond:Ltions (Olsnes, 5 S. & Eiklid, K. J. Biol. Chem. 255, 284-289 (1980)). In some cases the translation product was treated with protein A-Sepharose (Pharmacia, Sweden), which had previously been incubated with rabbit anti-B3 antiserum (lanes 3 and 4) or anti-ricin (lane 5). The adsorbed material was analyzed by lO S~S-PAGE. DT, translation product from pBD-l; B3-DT, trans-lation product from pB-B3-D1; ss-DT, translation product from pGD-2.
FIG. 2. Translocation to the cytosol of A-fragment with N-terminally added B3 oligopeptide. p~D-1 and pB-B3-Dl were 15 transcribed and translated in vitro. ~he corresponding trans-lation products (DT and B3-DT) were added to Vero cells grow-ing as monolayers in 24-well microtiter plates and kept at ~4C for 20 min in the presence of 10 ,uM monensin ~McGill, S., Stenmark, H., Sandvig, ~. & Olsnes, S.: EMBO J. 8, 2843-2848 20 ( 1989)). The cells were washed twice with Hepes medium and subsequently treated with 0.4 lug/ml TPCK (N-tosyl-L-phenyl-alanine chloromethyl ketone)-treated trypsin in Hepes medium containing lO ~M monensin for 5 min at 20C. The cells were washed and exposed to Hepes medium, pH 4.8, containing 10 mM
zS Na-gluconate to increase the buffering capacity at the low pH.
After 2 min at 37C, the cells were washed with Hepes medium, pH 7.4, and then treatPd with 3 mg/ml pronase in Hepes medium, pH 7O4~ containing 10 ~M monensin for 5 min at 37C. The cells, which were detached from the plastic by the treatment, 30 were recovered by centrifugation and washed once with Hepes medium containing l mM NEM (N-ethyl maleimide) and 1 mM PMSF
(phenylmethylsulfonyl fluoride). In some cases, (lanes 1-3 and 8-lO) the cells were lysed with Triton X-lOO in phosphate buffered saline containing l mM PMSF and 1 mM NEM, nuclei were 35 removed by centrifugation and the protein in the supernatant fraction was precipitated with lO~ (w/v~ trichloroacetic acid or immunoprecipitated with anti-B3 antibodies adsorbed to protein A-SepharosP. In other cases (lanes 4-7) the cells were treated with 50 ,ug/ml saponin in PBS containing l mM PMSF and : :: .

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W092/0~99 PCT/NO91/OOOg3 3 ~ 2 1 mM NEM to release translocated A fragment, and then theproteins both in the pellet and in ~he supernatant fractions were precipitated with trichloroacetic acid. ]:n all cases the precipitated material was analyzed by SDS-PAGE (13.5~ gel) 5 under non-reducinq conditions.
FIG.3. Translocation to the cytosol of diphtheria toxin with signal sequence. Lanes 1-4: l25I-labelled natural toxin (wt-DT, lane 1) and in vitro translated pGD-2 ([35S]methionine labelled toxin with signal sequence, ss-DT) were bound to Vero o cells and nicked on the cells (lanes 1 and 2). In lane 3 the cells were treated as in lane 2, except that 6 times more translation product was used and the cells were then exposed to pH 4.8 and pronase as in Fig. 2. The cells were lysed with Tri-ton X-100 and the nuclei were removed. The supernatants were incubated with protein A-sepharose that had been pre-incubated with rabbit anti-diphtheria toxin serum. The adsorb-ed material was analyzed by reducing (lanes 1 and 2) or non-reducinq (lanes 3 and 4) SDS-PAGE (10% gel). In lane 4 the pronase-treated cells were treated with 50 ~g/ml saponin and 20 the material released to the medium was analyzed directly.
Lanes 5-12: Translation products from pBD-1 (DT) and pGD-2 (ss-DT) were bound to Vero cells, nicked, exposed to pH 4.8 and then treated with pronase. The lysed cells were either analyzed with non-reducina SDS-PAGE (15~ gel) directly (lanes 25 5-8) or they were treated with saponin and the membrane pellets (l~nes 9 and 10) and the supernatant fractions (lanes 11 and 12) were analyzed separately.

Detailed Description . Diphtheria toxin is synthesized by pathogenic strains of Corvnebacterium diphtheriae as a single chain polypeptide.
The protein is easily split ("nicked") at a trypsin-sensitive site to yield two disulfide-linked fragments, A and B (Pappen-haimer, A.M., Jr. Annu. Rev. Biochem. 46, 69-94 (1977)).
The B-fragment ~37 kD) binds to cell surface receptors, whereas the A-fragment (21 kD) is an enzyme that is trans-located to the cytosol where it inactivates elongation factor 2 by ADP-ribosylation and thus blocks protein synthesis (Van Ness, B.G., Hovard, J.B. & Bodley, J.W. J. Biol. Chem. 255, . . .
.. ~, .. . ' . '- - ' W092/0~99 PCT/NO91/00093 208~3~2 6 ~`
10710-10716 (1980)). The translocation, which normally occurs across the limi-ting membrane of endosomes, is triggered by the low pH in the acidic vesicles (Draper, R.K. & Simon, M.I. J.
Cell Biol. 87, 849-854 (1980); Sandvig, K. & Olsnes, S. J.
S Cell Biol. 87, 828-832 (1980)). When cells with surface-bound toxin are exposed to acidic medium, translocation occurs from the cell surface (Sandvig, K. & Olsnes, S. J. Biol. Chem. 256, 9068-9076 (1981)). We have in the presented examples used this artificial system, because it enables us to distinguish 10 between translocated and non-translocated material (Moskaug, JØ, Sandvig, K. & Olsnes, S. JO Biol. Chem. 262, 10339-10345 (1987); Moskaug, JØ, Sandvig, K. & Olsnes, S. J. Biol. Chem.
2~3, 2518-2525 (1988)).
To avoid toxic effect on the cells by the diphtheria 15 toxin vec-tor, a mutant toxin was used which contains a triple mutation changing Glu14a, which is located in the enzymatica:Lly active site of the toxin, to Ser (Barbieri, J. T. & Collier, R.J. Infect. Immun. 55, 1647-1651 (1987)). The modified toxin has strongly reduced toxicity.

ExamPles We used two variants of the mutated toxin gene, one without (pBD-1) (McGill, S., Stenmark, H., Sandvig, K. &
Olsnes, S.: EMBO J. 8, 2843-2848 (1989)), and one with (pGD-2) 25 the natural 25 amino acids signal sequence (Fig. lA). In one case, a foreign oligopeptide, termed B3, was linked to the N-terminal end of the toxin to yield the plasmid pB-B3-D1.
The constructs, which were placed behind T3 or SP6 RNA-polymerase promotors, were transcribed and translated in vitro 30 (McGill, S., Stenmark, H., Sandvig, K. & Olsnes, S.:EMBO J. 8, 2843-2848 ~1989)). In each case a major band corresponding to the full-length protein and only traces of material of lower molecular weights were obtained (Fig. lB). Toxin with signal sequence (lane 7) or with B3 (lane 1) migrated, as expected, 35 slightly more slowly than toxin as such (lanes 2 and 6).
Furthermore, toxin with B3 was selectively precipitated with anti-B3 (lane 4), but not with a control serum (lane 5). ~roxin without B3 was not precipitated with anti-B3 (lane 3).
The dialyzed translation products were bound to Ve:ro ' -: ' ' ' ~ '' .
.

W092/0~99 PCT/NO91/00093 ~ 7 2~3~2 cells, nicked on the cells with low concentrations of trypsin, and then the cells were exposed to pH 4.8. Under these conditions part of the bound toxin was translocated to the cytosol and thereby became shielded against pronase added to 5 the medium (Moskaug, JØ, Sandvig, K. & Olsnes, S. J. Biol.
Chem. 263, 2518-2525 (1988)). In the case of diph-theria toxin as such, two fragments (MW 21 kD and 25 kD) w~re protected under these conditions (Fig. 2, lane 1), corresponding to the whole A-fragment (21 kD) and part of the B fragment (25 kD out o of total 37 kD). The interfragment disulfide was reduced, apparently upon exposure to the cytosol (Moskaug, JØ, Sandvig, K. & Olsnes, S. J. Biol. Chem. 262, 10339-10345 (1987)).

15 ExamPle 1 When the same experiment was carried out with toxin containing B3, two major fragments (25 kD and 22.5 kD) were protected in addition to small amounts of 21 kD fragment (lane 2). The latter probably represents A-fragment where B3 had 20 been cleaved off. When the exposure to low pH was omitted, no fragments were protected (lane 3). The 22.5 kD fragment was precipitated by anti-B3 (lane 9), but not with preimmune serum (lane 10). Protected A-fragment without the oligopeptide was not precipitated with anti-B3 (lane 8). The apparently higher 25 amount of protected A-fragment with B3 is due to more radio-activity incorporated, as B3 contains 3 methionines and the A-fragment alone 5.
When cells with translocated diphtheria toxin are treated with low concentration of saponin allowing cytoplasmic 30 marker enzymes to leak out of the cells without dissolving the membranes, the translocated A-fragment is released into the medium, whereas the B-fragment-derived 25 kD polypeptide remains associated with the membrane fraction (Moskaug, JØ, Sandvig, K. & Olsnes, S. J. Biol. Chem. 263, 2518-2525 (1988~;
35 Moskaug, JØ, Sletten, K., Sandvig, K. & Olsnes~ S. J. Biol.
Chem. 264, 15709-15713 (1989); Moskaug, JØ, Sandvig, K. &
Olsnes, S. J. Biol. Chem, 264, 11367-11372 (1989)). This indi-cates that the translocated A-fragment is fr~e in the cytosol, whereas the 25 kD polypeptide is inserted into the membrane.

W092~00099 PCT/NO91/00093 Also most of ~e8A~ragment containing B3 was released wi-th saponin ~lane 7) in the same way as normal A~fragment (lane 6), whereas the 25 kD fragment was associated with the membranes (lanes 4 and 5). Therefore, it appears that diph- , 5 theria toxin is able to translocate B3 (14 amino aclds) to the cytosol.

Example 2 To test if also a larger oligopeptide could be trans-o located, we chose toxin carrying its normal signal sequence (25 amino acids). As shown in Fig. 3, lane 2, this protein was nicked by trypsin into a 23O5 kD A-fragment and a 37 kD B-fragment. (In this experiment the toxin was only partially nicked. Partially nicked 12sI-labelled natural toxin is shown 5 for comparison in lane 1). When the toxin with signal sequence was bound to cells, nicked, and then exposed to pH 4.8, two fragments (23.5 kD and 25 kD) were protected against pronase (lane 8). Protected A fragment with uncleaved signal seguence is also shown in lane 3, where the material was precipitated 20 with an anti-diphtheria toxin serum which binds the whole toxin, the A-fragment, as well as whole B-fragment (see lanes 1 and 2), but not the 25 kD-fragment. When the pronase-treated cells were treated with saponin, the extended A-fragment was released to the medium (lanes 4 and 12), whereas the 25 kD
25 fragment remained in thie membrane fraction (lane 10).

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Claims

1. A method of introducing a peptide into the cytosol, characterized by linking the peptide to a bacterial or plant toxin, or a mutant thereof.

2. A method of preparing a vaccine, characterized by linking a peptide to a bacterial or plant toxin, or a mutant thereof to translocate the pep-tide into the cytosol for subse-quent presentation at the cell surface by Class I MHC antigens to elicit a Class I restricted immune response and to expand the relevant population of CD8+ T-lymphocytes.

3. The method according to claims 1 or 2, characterized by using a mutant of a bacterial or plant toxin which has been manipulated in such a way that it has lost its toxicity with-out having lost the ability to enter the cytosol and to carry additional peptide material into the cytosol.

4. The method according to claims 1 or 2-3, characterized by using a non-toxic mutant of diphtheria toxin or a related toxin such as ricin, abrin, modeccin, viscumin, volkensin, Pseudomonas aeruginosa exotoxin A, Shigella toxin, cholera toxin, E. coli heat labile toxin of pertussis toxin.

5. The method according to claims } or 2-4, characterized by using a non-toxic mutant of diphtheria toxin.

6. A vaccine, characterized by having been produced by a method according to claims 2-5.

7. The use of a vaccine according to claim 6 against viruses, intracellular bacteria and parasites, and against molecules associated with malignancies.