WO1997045144A1

WO1997045144A1 - Construction and use of genes encoding pathogenic epitopes for treatment of autoimmune disease

Info

Publication number: WO1997045144A1
Application number: PCT/US1997/010214
Authority: WO
Inventors: Leslie P. Weiner; Minnie Mcmillan
Original assignee: University Of Southern California
Priority date: 1996-05-29
Filing date: 1997-05-29
Publication date: 1997-12-04
Also published as: EP1015034A4; RU2248807C2; US20040071673A1; AU734633B2; CA2256577A1; NO985576D0; US20020141983A1; NO985576L; US6274136B1; AU3234297A; EP1015034A1

Abstract

The present invention relates to the application of genetic engineering to provide a treatment of autoimmune disease. This is achieved preferably through the introduction of one or more recombinant genes encoding self antigens which are the target of an autoimmune response. In particular the invention provides a method of designing and constructing a gene encoding an encephalitogenic epitope of proteolipid protein, and to the in vivo expression of the gene product by a recombinant retroviral vector. The expression and secretion of the encephalitogenic epitope ameliorates the histophathological and clinical characteristics of experimental autoimmune encephalomyelitis (EAE) in the mouse model for multiple sclerosis (MS).

Description

S P E C I F I C A T I O N

CONSTRUCTION AND USE OF GENES ENCODING PATHOGENIC EPITOPES

FOR TREATMENT OF AUTOIMMUNE DISEASE

Field of the Invention

This invention relates generally to the field of immunotherapy and to the

preparation and use of engineered cells having the ability to restore tolerance to self

antigens in patients suffering from autoimmune disease. More particularly, this invention

relates to the design and construction of a gene encoding an encephalitogenic epitope of

proteolipid protein (PLP), to methods of in vitro and in vivo expression of a PLP epitope,

to methods of in vivo secretion of a PLP epitope, and to methods of transferring the

partial PLP gene to a host to ameliorate the progression of an immune response to self

antigens derived from myelin proteins. Background of the Invention

The immune system can respond in two ways when exposed to an antigen. A

positive response leads to differentiation of T and B cells, antibody production and to

immunologic memory. A negative response leads to suppression or inactivation of

specific lymphocytes and to tolerance. Tolerance can be defined as the failure of an

organism to mount an immune response against a specific antigen. Normally, an

organism is tolerant of its own antigens.

Autoimmune diseases are thought to result from an uncontrolled immune

response directed against self antigens. In patients with multiple sclerosis (MS), for

example, there is evidence that this attack is against the white matter of the central

nervous system and more particularly to white matter proteins. Ultimately, the myelin

sheath surrounding the axons is destroyed. This can result in paralysis, sensory deficits

and visual problems. MS is characterized by a T cell and macrophage infiltrate in the

brain. Autoreactive myelin-specific T cells have been isolated from MS patients,

although T cells of the same specificity have been detected in normal individuals. J.M.

LaSalle et al., J. Immunol. 147:774-780 (1991), J.M. LaSalle et al., J. Exp. Med.

176:177-186 (1992), J. Correale et al., Neurologv.45: 1370- 1378 (1995). Presently, the

myelin proteins thought to be the target of an immune response in MS include myelin

basic protein (MBP), proteolipid protein (PLP), and myelin-oligodendrocyte glycoprotein

(MOG). Individuals who do not mount an autoimmune response to self proteins are

thought to have control over these responses and are believed to be "tolerant" of self

antigens. The evidence, therefore, that MS is caused by pathogenic T cells is necessarily

indirect, but the close resemblance which the characteristics of this disease bear to those of the murine model, experimental autoimmune encephalomyelitis (EAE), suggest that

MS is indeed caused by an aberrant immune response mediated by T cells.

The EAE mouse model for MS, the subject of intense and fruitful study for

several years, displays many of the same histopathological and clinical characteristics as

the relapsing remitting forms of MS. The T Lymphocyte in Experimental Allergic

Encephalomyelitis. Ann. Rev. Immunol. 8:579-621 (1990). EAE can be induced in SJL

mice by injection of mouse spinal cord homogenate (MSCH), MBP, PLP, by the

injection of synthetic peptides whose sequences correspond to the major encephalitogenic

epitopes of myelin basic protein, MBP 84-104, proteolipid protein, PLP 139-151, or by

adoptive transfer of activated CD4⁺ T_H1 but not T_H2 cells specific for encephalitogenic

epitopes. The major encephalitogenic epitopes of myelin-derived sequences in EAE, such

as MBP, can also activate human T cells of several different haplotypes including HLA-

DR2. R. Martin, et al., J. Exp. Med. 173:19-24 (1992). The experimental disease is

characterized by a relapsing-remitting course (R-EAE) of neurological dysfunction,

perivascular mononuclear infiltration and demyelination. CNS damage is probably

mediated by inflammatory cytokines which can activate additional monocytes and

macrophages non-specifically. J.E. Blalock, The Immune System. Our Sixth Sense. The

Immunologist, 2:8-15 (1994).

Although the initial attack in EAE can be induced by the administration of either

T cells specific for MBP or for PLP, close examination of reactivities of T cells in the

primary and subsequent relapses demonstrates the presence of T cells which interact with

specificities other than the inducing epitopes. This expansion of encephalitogenic

epitopes is termed "determinant spreading". S.D. Miller and W.J. Karpus, Immunology Today 15:356-361 (1994), P.V. Lehman, T. Forsthuber, A. Miller, and E.E. Sercarz,

Nature 358-155-157 (1992), H. Jiang, S-I. Zhang and B. Pernis, Science 256: 1213-1215

(1992). Antigen specific treatment would therefore, be expected to be more effective

when administered early in the course of the disease, before the onset of increasing

epitope complexity and eventual non-specific inflammation.

The goal of immunologic therapy is to restore tolerance without suppressing the

entire immune system which can lead to complications such as infection, hemorrhage,

and cancer. Drugs currently used to treat autoimmune diseases are non-specific

immunosuppressive agents, such as anti-inflammatory agents or drugs which can block

cell proliferation or depress proinflammatory cytokines. In general, these agents are

effective for limited duration and subject to devastating complications.

It is desirable to suppress the immune system in a more specific way to control

the response to self-antigens and theoretically "cure" the disease without down-regulating

the entire immune system. Several specific immunotherapies have been hypothesized

and tested in recent years, many of which are impractical or do not work in humans. For

example, high affinity peptides can be synthesized which interact with MHC class II

molecules and prevent the binding of encephalitogenic peptides, thereby preventing the

activation of pathogenic T cells. A. Franco et al., The Immunologist 2:97-102 (1994).

This approach is disadvantageous in that it is difficult to obtain effective concentrations

of inhibitor peptides in vivo. G.Y. Ishioka et al., J. Immunol. 152:4310-4319. In an

alternate strategy, peptides which are analogs of encephalitogenic sequences have been

shown to antagonize the T cell receptors of antigen-specific T cells, rendering them

unreactive, although the exact mechanism is at present unknown. S.C. Jameson et al., J. Exp. Med 177:1541-1550 (1993), N. Karin et al., J. Exp. Med. 180:2227-2237 (1994),

V.K. Kuchroo et al., J. Immunol. 153:3326-3336 (1994). Oral administration of myelin

has been tested and found to induce a state of immunological unresponsiveness thought

to be mediated by the induction of suppressor T cell or of anergy. H.L. Weiner et al.,

Annu. Rev. Immunol. 12:809-837 (1994), C.C. Whitacre et al.. J. Immunol.. 147:2155-

2163 (1991), SJ.Khoury et al.. J. Exp. Med. 176:1355-1364 (1992). This treatment has

been found to be efficacious for some but not all individuals. H.L. Weiner et al., Science

259: 1321 - 1324 ( 1993). Thus, it is evident that improvements are needed to treat MS and

other autoimmune disorders with an effective, immunospecific approach.

Summary of the Invention

The present invention addresses the disadvantages present in the prior art. In

general, the invention is based on the discovery that recombinant DNA technology and

cell transfer may be employed to restore tolerance to one's own tissues. The present

invention provides a means of preparing and constructing a gene, that when expressed

and secreted in vivo, can provide a means of halting the progression of an autoimmune

disease. In further aspects the invention provides a method to construct a gene encoding

a portion of a CNS protein, insert the gene sequence into a vector and transfect a cell line.

In further aspects, the invention provides a method to construct a gene encoding a portion

of a CNS protein, insert the sequence into a retroviral vector, and transduce a producer

fibrobiast cell line to generate supernatant containing the recombinant retrovirus.

Histocompatible fibroblasts are transduced with the recombinant retrovirus encoding a portion of the CNS protein and are delivered to animals. These fibroblasts continuously

secrete a CNS antigen in vivo but do not themselves produce viral particles.

In accordance with the present invention, we have used synthetic oligonucleotides

to construct a gene encoding a portion of the PLP protein, performed expression of the

DNA in combination with various expression vectors, and thereby evaluated expression

levels of the gene product in vitro and in vivo. After transduced histocompatible

fibroblasts that secrete the partial PLP protein are transplanted into EAE mice, the disease

disappears. The effect is the amelioration of both clinical symptoms and signs and

pathological findings.

In a preferred embodiment of the invention, the producer line PA317 is

transduced with the PLP retroviral vector to generate supernatant containing the

recombinant retrovirus. The producer cell line PA317 was developed by Dr. A. Dusty

Miller and has been extensively characterized and approved for human use by the FDA

for other clinical trials, such as for genetic diseases and cancer. Miller and Baltimore,

Mol. Cell Biol. 6:2895-2902 (1986), W.F. Anderson, Science 256:808-813.

Brief Description of the Drawings

FIGURE 1 is a map of the partial PLP gene showing the sequence of the gene product

and restriction sites.

FIGURE 2 is a map of the GlXSvNa vector illustrating restriction sites and functional

features. Figure 2b illustrates the entire DNA sequence of GlXSvNa.

FIGURE 3 outlines the method of constructing a GlXSvNa vector containing the PLP

gene insert.

FIGURE 4 shows the level of mRNA expressed in transfected and transduced SJL

fibrobiast cells as detected by reverse transcriptase PCR. Lane 1 is molecular weight

standards, Lane 2 is Negative control from mock transfection, Lane 3 is positive control-

PLP-gene plasmid, Lane 4 is cDNA from PLP-transfected SJL fibroblasts, Lane 5 is

cDNA from PLP transduced SJL fibroblasts.

FIGURE 5 demonstrates the level of PLP protein in the supernatants of transduced

fibroblasts as detected by ELISA.

FIGURE 6 demonstrates the level of B-Gal expression in transduced fibroblasts.

FIGURE 7 illustrates the clinical scoring system for chronic EAE. FIGURE 8 illustrates the histological scoring system for EAE.

FIGURE 9 illustrates the clinical assessment of EAE mice treated with retrovirus

transduced fibroblasts.

FIGURE 10a shows the pathologic assessment of brain and spinal cord of SJL mice

treated with retrovirus transduced fibroblasts, and 1 Ob is a summary of the pathologic

assessment of brain and spinal cord from Days 55-60 through days 90-95.

FIGURE 11 shows the histology of SJL mice with chronic EAE treated with retrovirus

transduced fibroblasts.

FIGURE 12 illustrates the results of proliferation assays using EAE mice treated with

PLP-expressing fibroblasts.

FIGURE 13 illustrates the results of proliferation assays with and without IL-2 using

EAE mice treated with PLP-expressing fibroblasts.

Detailed Description of the Invention

As indicated above, the present invention relates to the use of engineered cells to

restore tolerance to self antigens in patients suffering from autoimmune disease. The

engineered cells can be any mammalian cell. As used herein, the term "engineered" is intended to refer to a cell into which one or more recombinant genes, such as a gene

encoding an epitope of a self antigen, has been introduced.

A gene is a deoxyribonucleotide sequence coding for an amino acid sequence.

Recombinantiy introduced genes will either be in the form of a synthetic oligonucleotide,

a cDNA gene (i.e. they will not contain introns), a copy of a genomic gene sequence, or

a hybrid gene which is a fusion of two or more gene sequences. Optionally the gene may

be linked to one or more nucleotide sequence capable of directing expression of the gene

product. Sequence elements capable of effecting expression of a gene or gene product

include but are not limited to promoters, enhancer elements, transcription termination

signals, polyadenylation sites, a Kozak box sequence to ensure efficient translation, and

leader sequences. Optionally, the gene sequence can include restriction sites to enable

the insertion of additional gene sequences. Preferably, the gene will contain a leader

sequence to ensure the gene product is synthesized in the endoplasmic reticulum for later

constitutive secretion.

Recombinantiy introduced genes carried by the engineered cells can encode one

or more epitope, fragment, domain or mini-protein portion of a protein antigen.

Examples of suitable proteins from which an epitope, fragment, domain, or mini-protein

may be derived include but are not limited to myelin proteins, acetylcholine receptor,

TSH receptor, and collagen.

It is believed that protein self-antigens which are the target of an autoimmune

response are highly conserved both among and between species. Thus, although the

invention will primarily be used to treat humans it can also be used to treat animals.

Examples of T cell mediated autoimmune diseases that may be treated using the invention include but are not limited to multiple sclerosis, myasthenia gravis, systemic

lupus erythematosus, psoriasis, juvenile onset diabetes, rheumatoid arthritis, thyroid

disease and chronic inflammatory demyelinating polyneuropathy (CIDP).

Expression vectors are generally deoxyribonucleotide molecules engineered for

controlled expression of one or more desired genes. The vectors may comprise one or

more nucleotide sequences operably linked to a gene to control expression of the desired

gene or genes. There are an abundance of expression vectors available and one skilled

in the art could easily select an appropriate vector. In addition, standard laboratory

manuals on genetic engineering provide recombinant DNA methods and methods for

making and using expression vectors. Optionally, the vector may encode a selectable

marker, for example, antibiotic resistance.

The gene can be inserted into the mammalian cell using any gene transfer

procedure. Examples of such procedures include but are not limited to, RNA viral

mediated gene transfer such as retroviral transduction, DNA viral mediated gene transfer,

electroporation, calcium phosphate mediated transfection, microinjection or liposome

mediated gene transfer. The type of procedure required to achieve an engineered cell that

secretes the desired gene product will depend on the nature and properties of the cell.

The specific technology for introducing such genes into such cells is generally known

and well within the skill of the art.

The examples which follow illustrate the design and construction of a portion of

the PLP gene, in vitro and in vivo expression of the PLP gene product, and the in vivo

effects of the PLP gene product. The following examples are presented to illustrate the invention, and are not

intended to limit the scope thereof.

EXAMPLE 1

DESIGN AND CONSTRUCTION OF THE PLP GENE

In SJL/J mice, the encephalitogenic epitope of PLP comprises amino acids 139-

151. N Takahashi et al., £ejl 42:139-148 (1985), K Sakai et al., J. Neuroimmunol. 19:21-

32 (1988), D.H. Kono et al., J. Exp. Med. 168:213-227. The vector in the present

invention is designed in order that the gene product encoded by it be constitutively

secreted from fibroblasts. Since the complete PLP protein is a hydrophobic

transmembrane protein (H-J. Diehl, M. Schaich, R-M. Buszinski and W. Stoffel, PNAS

U.S.A. 83:9807-981 1 (1986)), with the encephalitogenic epitope being extracellular, a

plasmid encoding amino acids 101-157 and additional amino acids required for secretion

was constructed. This sequence is hydrophilic in character.

1. Oligonucleotide synthesis and construction of the PLP pRc/CMV vector

Oligonucleotides can be synthesized manually, e.g., by the phospho-tri-ester

method, as disclosed, for example in R.L. Letsinger, et. al., J. Am. chem. Soc. 98:3655

(1967), the disclosure of which is incorporated by reference. Other methods are well

known in the art. See also Matteucci and Caruthers, J. Am. Chem. Soc. 103:3185 (1981),

the disclosure of which is incorporated by reference. Preferably, however, the desired gene sequence can be made by automated

synthesis of individual ohgonucleotides at .2μM concentrations. For PLP amino acids

101 -157, DNA syntheses were performed on a Perkin Elmer/Applied Biosystems

Division Model 394 DNA synthesizer using cyanoethyl-protected phosphoramidites. The

dimethoxytrityl (DMT) group was not removed from the 5'hydroxyl group to allow for

purification. After normal cleavage from the resin using concentrated ammonium

hydroxide and deprotection at 55 °C for 16 hours, the ohgonucleotides were purified

using oligonucleotide purification cartridges (OPC) according to the manufacturer's

instructions (Applied Biosystems Inc.). Five ohgonucleotides of the following sequences

were synthesized:

OLG1 5' - CGGCGACTACAAGACCACCATCTGCGGCAAGGGCCTGAGCGC

AACGGTAACAGGGGGCCAGAAGGGGAGGGGTTCCAGAGGCCA

ACATCAAGCTCATTCTCTCGAGC-3',

OLG2 5' - GAGCTTGATGTTGGCCTCTGGAACCCCTCCCCTTCTGGCCCCCT

GTTACCGTTGCGCTCAGGCCCTTGCCGCAGATGGTGGTCTTGTA

GTCGCCGGGCC-3',

OLG3 5' - GGGTGTGTCATTGTTTGGGAAAATGGCTAGGACATCCCGACAA

GTTTGTGGGCATCACCTATGCTAGCCTTAAGTAGGATCCTTGAA

TAGGTA-3',

OLG4 5' - AGCTTACCTATTCAAGGATCCTACTTAAGGCTAGCATAGGTGA

TGCCCA-3',

and OLG55'- CAAACTTGTCGGGATGTCCTAGCCATTTTCCCAAACAATGACA

CACCCGCTCGAGAGAAT-3'.

Each purified oligonucleotide was dried under vacuum, washed with 1 ml of

sterile double distilled water and then concentrated to dryness under vacuum (Speed vac

evaporator; Savant Inc.). 80pM of each oligomer was kinased at 37°C for 1 hour by

resuspending in 56.6μl of IX kinase buffer (Polynucleotide Kinase Buffer; Boehringer

Mannheim, Indianapolis, IN) containing 10 units of polynucleotide kinase (Boehringer

Mannheim) and 100μM of ATP. The individual ohgonucleotides were combined in the

presence of 2X SSC (0.03M Sodium Citrate, pH 7.0, and 0.3M NaCl) in a PCR tube with

their respective complementary oligomer partners for annealing. Each annealed set

measured 200μl in volume. Oligomer OLG1 was annealed with OLG2, and oligomers

OLG4 and OLG5 were annealed with OLG3. Annealing was performed in a Perkin-

Elmer 9600 Thermocycler, programmed as follows: 1)99.9° for 2 minutes, and 2) 99.9°

to 4° in 15 minutes. During the temperature descent to 4°C, when the thermocycler

temperature reached 37°C, the solution containing the oligomer duplex OLG1 and OLG2

was combined with the solution containing the oligomers OLG3, OLG4, and OLG5. The

descent cycle was then continued until it reached 22 °C. Subsequently, 5 units (5μl) of

T4 ligase (Boehringer Mannheim, Indianapolis, IN) and 45μl of manufacturer's 10X T4

DNA ligation buffer (Boehinger Mannheim, Indianapolis, IN) was added, and ligation

proceeded overnight at 10 °C.

The ligated DNA was precipitated with 2 volumes of 100% ethanol and incubated

at -70°C for 1 hour. The precipitate was centrifuged for 30 minutes at 17000 x g at 4°C. The supernatant was discarded and pellet was washed with 1 ml of 70% ethanol and

centrifuged for 10 minutes at 17000 x g at 4°C. The DNA pellet was dried under vacuum

(Speed vac evaporator; Savant Inc.) and resuspended in 45μl sterile double distilled

water.

DNA of the correct molecular weight was isolated by electrophoresis. 5μl of lOx

loading buffer (6.25g Ficoll and 0.93g Disodium EDTA/25ml 10% SDS, Orange G,

Xylene Cyanole, and Bromophenol Blue) was added to the sample and loaded onto a 14.5

cm x 16cm x 0.15mm urea/acrylamide gel (7M urea/8% acrylamide with 1.1% Bis).

TBE (89mM Tris, 89mM Boric acid, and 2mM EDTA pH8.0) was used as both gel and

electrophoresis buffer. The sample was electrophoresed at 35mA until the Orange G dye

line had migrated within 1 cm of the bottom of the gel. The acrylamide gel was washed

twice with water for 5 minutes. After the last wash, the gel was incubated for 3 minutes

in a 500 ml solution containing lOul of lOmg/ml of ethidium bromide, and visualized

under a UV-Iight source. The band corresponding to the ligated DNA was excised and

cut into small pieces for electroelution in an IBI electroelutor apparatus (Model UEA:

International Biotechnologies Inc., New Haven, CT).

For electroelution, the salt trap of the apparatus was filled with 125μl of 7M

sodium acetate/bromophenol blue dye solution. The buffer chamber was filled with 1/2X

TBE. The sample was electroeluted for 1 hour at 85V. After removing the eluted DNA,

the sample well was washed with 1/2X TBE and combined with the initial eluate. The

eluted DNA was then precipitated overnight at -70 °C with 2 volumes of 100% ethanol.

The precipitate was pelleted, washed as previously described, and resuspended in 15ul

of sterile double distilled water. Preceding the ligation of the eluted partial PLP gene to the pRc/CMV vector

(Invitrogen, San Diego, CA), the pRc/CMV vector construct was cut with the restriction

endonucleases Apa I and Hind III according to the Manufacturer's instructions

(Boehringer Mannheim, Indianapolis, IN). The resuspended PLP gene construct was

then added to a 5μl mixture containing 0.3μg of pRc/CMV cut vector (2μl), 1 unit T4

ligase (lμl) (Boehringer Mannheim, Indianapolis, IN), and 2μl of Manufacturer's 10X

T4 DNA ligation buffer (Boehringer Mannheim, Indianapolis, IN). The ligated vector

was then transformed into the competent cell line AG1.

Transformation proceeded by combining the ligation mixture with the AG1 cells

and incubating it on ice for 20 minutes. The cell/vector mixture was then incubated at

42° for 2 minutes and plated overnight onto a Luria Broth agar (LB; Biol 01, Vista, CA)

plate, supplemented with 80 mg/ml of ampicillin (Sigma, St. Louis MO). Colonies were

screened for the correct sequence vector by first isolating the plasmid DNA and then

sequencing the DNA.

To isolate the plasmid, a commercially available plasmid purification kit, Wizard

Minipreps (Promega, Madison, WI) was used. Colonies were picked from the LB/Amp

plates and grown for 3.5 hours in 5 ml of LB medium (BIO 101, Vista, CA)

supplemented with 80mg/ml of ampicillin (Sigma, St. Louis, MO). 3 ml of the medium

was centrifuged at 17000 x g at room temperature, for 1 minute to pellet the cells.

Isolation of the plasmid proceeded according to the Manufacturer's instructions, lμg of

the isolated DNA was used for sequencing.

The oligonucleotide sequence can be checked by methods well known in the art,

such as that described by Sanger et. aLPNAS U.S.A. 70:1209 (1973) or by the Maxam- Gilbert method, Meth. Enzymology. 65:499 (1977), the disclosures of both of which are

incorporated herein by reference. Preferably, the plasmid can be sequenced using an

automated DNA sequencer. For the PLP pRc/CMV construct, the plasmid was

sequenced using automated fluorescent DNA sequencing procedures (Perkin

Elmer/Applied Biosystems Ine, Foster City, CA) using the following primers:

GATTTAGGTGACACTATAG and TAATACGACTCACTATAGGG. These primers

primed off the vector, which flanked the Kozak and "stop" site of the total construct.

Figure 1 shows a map of the partial PLP gene showing the sequence of the gene product

and restriction sites. At the 5' end of the construct we had previously inserted a

hydrophobic leader sequence from the MHC class I L^d gene to enable the gene product

to be synthesized in the endoplasmic reticulum (ER) for later constitutive secretion. Linsk

et al. J.Exp. Med. 164:794-813 (1996). In addition, a lysine codon at the 3' end was

added to ensure that the protein could not be retained in membrane. A Kozak box was

included in the construct to ensure efficient translation. Restriction sites Afl II and

BamHI were included in the construct to allow for insertion of further epitopes.

EXAMPLE 2

IN VITRO EXPRESSION OF THE PLP PROTEIN

The following experiments were performed in order to demonstrate that the PLP

vector encodes a protein which is constitutively secreted. Specifically, the mRNA levels

of PLP were evaluated in SJL fibrobiast cells transfected with the pRc/CMV-PLP vector,

and mRNA and protein levels of PLP were evaluated in SJL fibrobiast cells transfected

with the pGlPLPSvNa vector. 1. Establishment of Fibrobiast Cultures

Syngeneic fibroblasts (derived from SJL mice) were obtained from Dr. G.

Dveskler (Uniformed Services University, Bethesda, MD) and expanded at 37°

incubation using DMEM growth medium, supplemented with 5% glutamine and 10%

FCS. The cells were harvested and frozen at 1 x 10⁷ cells per vial, and aliquots were

quality control tested for mycoplasma, sterility and viability.

2. Retroviral Constructs

A recombinant retroviral vector in which exogenous genes are inserted into a

retroviral vector was constructed. The cloning strategy was to construct a pGlXSvNa

vector (W. French Anderson, University of Southern California) containing the PLP

insert from pRc/CMV-PLP. The pGlXSvNa vector, like most retroviral vectors used in

preclinical and clinical trials, is derived from the Moloney murine leukemia retrovirus

(Mo-MLV). Rosenberg et al., N. Eng. J. Med. 323:570-578 (1990), Culver et al.,

Science 256: 1550-1552 (1992). The GlXSvNa vector is a 5865 bp vector whose map,

functional features and complete DNA sequence are shown in Figures 2a and 2b. Figure

3 illustrates the procedure for constructing the pGlPLPSvNa vector. Essentially, the

pRc/CMV-PLP vector was digested with BstEII/Hindlll and PLP encoding fragment was

isolated by gel electrophoresis. After electroelution, Hindlll/Notl adapters (Stratagene,

La Jolla, CA) were ligated into the Hindlll site of the eluted fragment. A Notl digestion

was performed to generate Notl ends. A Notl digest was performed on pGlXSvNa and

the 5865 bp fragment was isolated, electroeluted, and a CIAP (Calf intestine alkaline

phosphatase treatment) was performed on the fragment ends. The Notl site of the insert was ligated into the Notl site of the vector. BstEII ends of the insert and Notl site of the

vector were Klenowed. A blunt end ligation is performed to close the vector. HB101

cells were transformed with ligation mix and restriction analysis was performed to

determine which vectors contain insert and the insert orientation. The recombinant

retroviruses are non-replicating and incapable of producing infectious virus.

3. Retroviral vector supernatant

To prepare supernatant containing PLP-recombinant retrovirus, the PLP-

transduced retroviral packaging cell line PA317 was grown in 4 ml of appropriate culture

medium in a T25 flask (Corning, Cambridge, MA). Retroviral vector supernatant is produced by harvesting the cell culture medium when cells were 80-90% confluent, and

stored in 1 ml aliquots at -70C°.

The following tests were performed on the PLP cell line and/or the vector supernatants:

(1 ) The viral titer is determined using 3T3 cells. Viral preparations with titers

greater than 5 X 10⁴ colony forming units/ml are used.

(2) Sterility of the producer cell line and the supernatant is assured by testing for

aerobic and anaerobic bacteria, fungus and mycoplasma.

The PLP-vector preparations from PA317 can be extensively tested to assure that

no detectable replication competent virus is present. This is particularly relevant to the

embodiment of the invention wherein the invention is used to treat humans. Tests on

both the viral supernatant and on the transduced fibroblasts can be performed to determine if there is replication competent virus present. The following tests can be

performed on the producer cell line and/or the viral supernatant:

greater than 5 X 10⁴ colony forming units/ml are used.

(2) Southern blots are run on the producer cell line to detect the partial PLP

gene.

(3) PLP production by the producer cell line is measured and should be

significantly above baseline control values, as determined by ELISA assay.

(4) Sterility of the producer cell line and the supernatant is assured by testing for

aerobic and anaerobic bacteria, fungus and mycoplasma.

(5) Viral testing is performed including: MAP test, LCM virus, thymic agent,

S + L-assay for ecotropic virus, S + L assay for xenotropic virus, S + L-assay for

amphotropic virus and 3T3 amplification.

(6) Electron microscopy is performed to assure the absence of adventitious

agents.

Following the introduction of the gene into fibroblasts, the following tests are

performed on the fibroblasts prior to administration to patients.

(1) Cell viability is greater than 70% as tested by trypan blue dye exclusion.

(2) Cytologic analysis is performed on over 200 cells prior to infusion to assure

that tumor cells are absent.

(3) Sterility is assured by testing for aerobic and anaerobic bacteria, fungus and

mycoplasma.

(4) S + L-assay including 3T3 amplification must be negative. (5) PCR assay for the absence of 4070A envelope gene must be negative.

(6) Reverse transcriptase assay must be negative.

(7) Southern blots run on the transduced fibroblasts to assure that intact provirus

is present.

(8) PLP protein assay to assure the production of PLP protein.

4. Transfection of fibroblasts

Prior to the transfection of the SJL fibroblasts, highly purified PLP-pRc/CMV

vector was isolated from the transformed AG1 cells. Large scale purification was

performed by using a commercially available kit and CsCl gradient banding. Initial

purification was accomplished using a Wizard Megaprep Kit (Promega, Madison, WI).

A 1000ml culture of transformed AG1 cells, grown overnight in LB/Amp at 37°C, was

pelleted and the plasmid DNA isolated according to the Manufacturer's instructions. The

isolated DNA, which was suspended in 3 ml of TE buffer (lOmM Tris-HCl, pH 7.4, and

ImM disodium EDTA, pH, 8.0) was further processed by CsCl gradient banding. A

modified CsCl banding of the DNA was performed based on procedures found in

"Current Protocols in Molecular Biology, Vol 1 " (Greene Publishing Associates and

Wiley-Interscience).

After the DNA band was extracted from the ultracentrifuge tubes, ethidium

bromide was removed from the sample by washing it with 3 volumes of SSC saturated

isopropanol. The wash was repeated until the aqueous layer appeared clear. CsCl was

removed by precipitation. 2 volumes of 0.2M NaCl/TE and 2 volumes of 100% ethanol

(relative to the combined total volume of DNA solution and 0.2M NaCl/TE) were added to the sample, mixed and placed on ice for 10 minutes. The precipitated DNA was

pelleted by centrifugation at 10000 x g for 10 minutes at 4°C. The pellet was washed

with cold 70% ethanol, recentrifuged at 10000 x g for 10 minutes at 4 °C, and dried under

vacuum (Speed vac evaporator; Savant Inc.). The purified DNA was resuspended with

double-distilled sterile water and utilized in the transfection process.

l est SJL fibroblasts were transfected using LipofectAMINE Reagent (Life

Technologies Inc./Gibco BRL) according to the manufacturer's instructions. Control SJL

fibroblasts underwent the same procedure without the presence of a DNA construct. 3μg

of CsCl purified PLP-pRc/CMV plasmid and 25μl of Lipofectamine were used for

transfection. Approximately 3 X 10⁵ SJL cells, seeded overnight into 25cm ²culture

flasks (Corning Costar Corp., Cambridge, MA.) and grown at 37° with 5% C0₂ in 5ml

of DMEM culture medium (Dulbecco's Modified Eagle's Medium (Irvine Scientific,

Santa Ana, CA), supplemented with 5% glutamine, 10% Fetal Calf Serum, 25 Units/ml

of penicillin G sodium, and 25μg/ml of streptomycin sulfate, were washed with 3ml

serum free HL-1 medium (Hycor Biomedical Inc., Irvine, CA). After the

DNA/lipofectamine complexes were incubated with cells for 6 hours at 37° with 5% Co₂

1 ml of DMEM was added to the flasks. The flasks were incubated overnight at 37° with

5% C0₂ The medium was replaced with 5ml of fresh DMEM the next morning. 36

hours after the end of the transfection period, the medium was replaced with 5ml of

DMEM containing 900μg of G418 (Life Technologies Inc./Gibco BRL)/ml of medium.

The test cells were grown in the presence of 900μg of G418 of medium until all the

control cells had died; and no more cell death could be observed in the test sample flask. The G418 concentration was then reduced to 600μg/ml of culture medium for duration

of cell culturing procedures.

5. Transduction of Fibroblasts

Retroviral constructs containing a neo-selectable marker together with either the

PLP gene or the Lac-z gene were used to transduce fibroblasts. Transduction with the

retrovirus was performed on healthy cells (90% viable, as determined by trypan blue

staining). 2 X 10⁶ cells were plated in 0.5 ml DMEM- 10 media (DMEM media

supplemented with 10% fetal calf serum, 2 mM L-glutamine, 50 U/ml penicillin G, 50

mg/ml streptomycin in one well of a 24- well plate (Falcon, Franklin Lakes, NJ). Cells were placed in the incubator and allowed to settle (37°, 5% CO₂). After cells had settled,

1 ml of retroviral supernatant and polybrene (Sigma, St. Louis, MO) (final concentration

l Oμg/ml) was added to the well. Cells were incubated as above for 2.5 hours without

shaking. After 2.5 hours, cells were transferred to a T25 flask and DMEM- 10 media was

added to a total volume of 8 ml. Selection media (culture media comprising DMEM- 10

supplemented with 900 μg/ml G418 (Gibco, Grand Island, NY) was added on the third

day after transduction. The G418 concentration was then reduced to 600μg/ml of culture

medium for the duration of cell culturing procedures.

6. mRNA expression analysis

mRNA isolation was performed using aseptic techniques, RNAse free supplies,

and DEPC (Diethylpyrocarbonate) treated solutions. 4 X 10⁶ experimental and control

SJL cells were washed twice with cold Phosphate-buffered saline, resuspended in 200μl cell lysis mix (lOmM TRIS pH 7.5, 0.15M NaCl, 1.5mM MgCl₂, 0.65% NP 40),

vortexed, and centrifuged at 17000 x g at 4° for 5 minutes. The supernatant was

transferred to a tube containing 200μl of urea mix (7M urea, 1% SDS, 0.35M NaCl,

lOmM EDTA, and lOmM Tris-HCL, pH 7.5) and 400μl of phenol :chloroform;isoamyl

alcohol (25:24:1). The solution was vortexed and centrifuged for 1 minute at 17000 x

g. This procedure was repeated twice using the aqueous layer and then transferred to a

tube containing 400μl of phenol and washed as before. The aqueous layer was

transferred again to another tube, and precipitated with 1ml of 100% ethanol overnight

at -20°C. The precipitated RNA was washed with 1ml 70% ethanol. After the ethanol

was discarded, the pellet was dried under vacuum. Iμg of the RNA was used for RT-

PCR analysis.

RT-PCR was performed using a commercially available kit, GeneAmp RNA PCR

Kit (Perkin Elmer/ABI) according to the Manufacturer's instructions. The following

primers were used to amplify the cDNA: 5^*-GCGACTACAAGACCACCATCT-3' and

5'-TAAGGCTAGCATAGGTGATG-3'. The PCR products were electrophoresed on a

1.5% agarose (SeaKem GTG; FMQ/TAE gel with lμl of lOmg/ml of ethidium

bromide/ml of agarose solution. The gel was electrophoresed using TAE buffer at a

constant 40mA. Electrophoresis was continued until the molecular weight marker bands

had separated adequately enough, to verify the PCR products' approximate molecular

size. The DNA band of interest was then excised and gel purified, using the

commercially available MERmaid Kit (Bio 101, Vista, CA), according to the

Manufacturer's instructions. The purified DNA was then sequenced by automated

Fluorescent DNA sequencing procedures (Perkin Elmer/ABI, Foster City, CA). Figure 4 is an agarose gel showing PLP-specific RT-PCR products. The data

illustrates that mRNA is present in both PLP-transduced and PLP-transfected cells. The

correlation between mRNA and secreted protein remains to be determined since peptide

concentration does not necessarily correspond to the level of mRNA.

7. Protein Expression Analysis

The in vitro qualitative expression of the proteins encoded by the PLP gene was

detected immunologically by ELISA. Undiluted supernatants from cultures of fibroblasts

transduced with the PLP gene were tested. Wells of 96 microtiter plate were coated with

the supernatants. Primary anti-PLP-antibody 4E 10 139- 151 , from Dr. M. Lees (Harvard),

is specific for PLP 139- 151 and was added to wells as undiluted hybridoma supernatant

followed by horseradish peroxidase (HRP)-conjugated goat anti-mouse secondary

antibody in a concentration of 1 :500. The plate was developed and analyzed at 490 nm

on a microplate reader. Figure 5 illustrates the results of ELISA assays on transduced

fibrobiast supernatants. Samples 1 and 2 were PLP (amino acids 139-151) and HIV

gpl20 peptides used at a concentration of 5ug/ml. This experiment illustrates that the

transduced PLP-transduced fibroblasts do produce and secrete the partial PLP protein.

EXAMPLE 3

IN VIVO EFFECTS OF THE PLP PROTEIN

Critical to the success of this invention in the embodiment of this example is the

ability to deliver genetically manipulated fibroblasts to patients so that the cells survive in sufficient numbers and for long periods of time, in order that continuous secreted

antigen may be provided to the patient.

To assess the fate of transplanted transduced fibroblasts, SJL fibroblasts

transduced with retrovirus encoding B-galactosidase were injected subcutaneously

between the shoulders of SJL mice. All mice were female mice of the SJL strain between

6-8 weeks old and were obtained from Jackson Labs. Animals were housed and

maintained according to NIH guidelines (National Research Council, 1986). These

fibroblasts survived in large numbers after 60 days. Fibroblasts injected into the footpad

or intramuscularly could not be detected at eight days.

1. In Vivo fate B-gal transduced cells

The activity of the B-Galactosidase marker was evaluated using two groups of

eight normal mice. Two mice were injected subcutaneously on the back, two mice were

injected intramuscularly and two mice were injected in the footpad with Lac-Z

transduced cells. One animal was injected with fibroblasts transduced with neo-marker

only, and the last mouse was injected with untransduced fibroblasts. After harvesting and

washing, the different cell lineages were suspended in a concentration of 10⁷ cells in .2

ml of Hank's PBS and slowly injected using a 25 gauge needle at different sites.

Animals were sacrificed at 10 and 15 days post treatment and injection sites were

submitted to histochemical study. Pieces of tissue were fixed in 4% paraformaldehyde

for one hour, washed in PBS three times and then kept in 8.4% acrylamide solution

overnight. The next morning tissues were embedded in acrylamide which after hardening

were cut and frozen. The frozen sections were done in lOum by cryostat and stained with 1 ml of 5-Bromo-4-chloro-3-indolyl-B-d-galactopyranoside (X-Gal) in PBS. The X-Gal

was dissolved in DMSO at 40mg/ml and then added to the reaction mixture. Incubation

was for 14-18 h at 37°. Figure 6 illustrates B-Gal expression in transduced fibroblasts

60 days in vivo. There was no evidence of an inflammatory response, suggesting that the

retrovirus used to transduce syngeneic fibroblasts, does not evoke an immune response

or rejection process.

2. Effect of PLP in normal SJL mice

Another important aspect of this invention in the embodiment of this example is

determining whether transduced fibroblasts secreting PLP actually produce EAE in

normal animals. To test this, 10⁷ PLP-secreting SJL fibroblasts were injected into 12

normal SJL mice. Six animals had fibroblasts placed subcutaneously and six animals had

fibroblasts injected intraperitoneally. Animals were sacrificed at day 16 and showed no

evidence of inflammatory disease or EAE. Figure 7 illustrates the clinical scoring system

for chronic EAE. Y-A Lu et al., Mol. Immunol.. 28:623-630 (1991), J. Williamson et al.,

J. Neuroimmunol. 32: 199-207 (1991). In the EAE model for multiple sclerosis, using

spinal cord homogenates plus adjuvant, inflammation in the CNS can be seen by day 14.

In this study, normal animals injected with PLP-secreting SJL fibroblasts did not show

any signs of clinical disease even at day 60. In addition, the animals did not show any

histologic evidence of inflammation in the CNS at day 60. Figure 8 illustrates the

histological scoring system for EAE. J. Govemman et al., Cell 72:551-560 (1993). 3. Clinical and histological assessment of acute EAE mice treated with retrovirus transduced fibroblasts.

Six week SJL mice were infected with mouse spinal cord homogenate (MSCH)

in complete Freund's Adjuvant (CFA) and with MSCH in incomplete Freund's Adjuvant

IFA, seven days later. J. Immunol. 144:909-915 (1990). The initial EAE attack was

observed on days 14-18, with full recovery by 21. Ninety-five percent of animals showed

clinical evidence of an acute attack and these were given either 10⁷ PLP secreting SJL

fibroblasts or control fibroblasts on day 21. Animals not showing clinical disease were

eliminated from the experiment. Figure 9 illustrates the clinical assessment of EAE mice

treated with retrovirus transduced fibroblasts. Animals receiving the PLP secreting

fibroblasts had a marked reduction of clinical signs and had dramatic reduction in

inflammatory cells, particularly in the brain. Figure 10a illustrates the pathologic

assessment of brain and spinal cord of SJL mice treated with retrovirus transduced

fibroblasts. Figure 10b is a summary of the pathologic assessment of brain and spinal

cord from days 55-60 and 90-95. Histological assessment of EAE Grades in Brain and

Spinal Cord were performed following the preparation of hematoxylin and eosin stained

sections.

4. Clinical and histological assessment of chronic EAE mice treated with retrovirus transduced fibroblasts.

150 mice were inoculated with MSCH in CFA. A second immunization was

given 7 days later. A.M. Brown and D.E. McFarlin, Laboratory Invest. 45:278-284

(1981). On day +14 to 16, 113 animals developed clinical disease lasting 3-4 days. These

positive animals were separated for subsequent experiments and had their first relapse on day +55 to 60, with 100 animals becoming sick. These were again separated and on day

+ 137, 67 had a relapse. Eight days after relapse, animals were each transplanted with 10⁷

fibroblasts and then sacrificed 18 to 23 days later. Four different types of fibroblasts

were used, those transduced with retrovirus encoding PLP, encoding B-galactosidase and

encoding neo-selectable marker as well as untransduced cells. Figure 11 shows the

histology of SJL mice with chronic EAE treated with retrovirus transduced fibroblasts.

There were no animals receiving PLP secreting fibroblasts with 2+ to 3+ inflammation.

5. Peripheral immune status of treated mice v. control EAE mice.

Spleen cells from our EAE control mice and from four EAE mice which had been

treated with fibroblasts expressing the PLP protein were used in proliferation assays, in

which they were incubated with 40μM PLP peptide 139-151 or 40μM HIV gpl20

peptide 308-322 for 4 days and then pulsed with ³H-thymidine for 24 hours.

Briefly, animals were sacrificed by CO₂ asphyxiation. Spleen cells were dispersed

to single cell suspensions in RPMI 1640 by passing through a size 60 mesh, and washed

once before being cultured (8 x 10⁵ per well) in 0.2 ml of HL-1 medium (Hycor

Biomedical, Irvine, CA), supplemented with 2mM glutamine, lOOU/ml penicillin, lOOμg

streptomycin either alone or with 40μM of peptide in 96-well tissue culture plates for 4

days at 37°C with 5% CO₂. PLP peptide 140-151 and MBP peptide 89-101 were used

for antigen-specific proliferation while HIV gpl20 peptide 308-322 was used as negative

control. Where indicated, some wells also contained 1 OU/ml of recombinant mouse IL-2

(Boehringer Mannheim, Indianapolis, IN). During the last 18-24 h of culture, each well

was pulsed with lμCi of ³H-thymidine (ICN, Irvine, CA), harvested onto 'Xtal Scint' glass fiber filters (Beckman, Fullerton, CA) and counted using a Beckman LS6000

Scintillation counter. Thymidine incorporation values (experimental counts per minute -

background counts per minute) were calculated and represent means of triplicate cultures

± standard deviation.

The results are shown in Figure 12 and suggest that PLP specific proliferative

responses are reduced significantly in EAE mice which have received PLP expressing

fibroblasts.

Figure 13 illustrates the same experiment as in Figure 12 but with the addition of

mouse IL-2 (1 OU/ml) for 5 days. These results illustrate that the mechanism by which

the PLP specific proliferative responses are reduced significantly may suggest the

possibility of deletion of T cells rather than anergy because these lymphocytes do not

respond to IL-2.

Although the mechanism by which the present invention acts to restore tolerance

in individuals suffering from T-cell mediated autoimmune disease is not entirely

understood, the benefits of the treatment are clearly advantageous over alternative

treatments. The method is a genetic approach to immunospecifically silence pathogenic

T-cell responses and does not down-regulate the entire immune system. In the case

where an individual with a T-cell mediated autoimmune disease exhibits pathogenic T-

cells of multiple specificities, the invention may easily be adapted to target those

specificities. For example, DNA encoding multiple self-antigenic epitopes may be

introduced into the patient's cells. The invention is also advantageous in that the reagents

can easily be made or obtained in sufficient quantity to carry out the invention. The present invention is not to be limited in scope by the exemplified

embodiments disclosed herein which are intended as illustrations of single aspects of the

invention, and clones, DNA or amino acid sequences which are functionally equivalent

are within the scope of the invention. Various modifications of the invention, in addition

to those shown and described herein, will become apparent to those skilled in the art from

the foregoing description. Such modifications are intended to fall within the scope of the

appended claims.

Various publications are cited herein that are hereby incorporated by reference in

their entireties.

SEQUENCE LISTING

(1) GENERAL INFORMATION:

(i) APPLICANT: Weiner, Leslie P.

McMillan, Minnie (ii) TITLE OF INVENTION: Construction and Use of Genes Encoding Pathogenic Epitopes For Treatment of Autoimmune Disease (iii) NUMBER OF SEQUENCES: 2 (iv) CORRESPONDENCE ADDRESS:

(A) ADDRESSEE: Kaye, Scholer, Fierman, Hays & Handler LLP

(B) STREET: 1999 Avenue of the Stars

(C) CITY: Los Angeles

(D) STATE: California

(E) COUNTRY: USA

(F) ZIP: 90067

(v) COMPUTER READABLE FORM:

(A) MEDIUM TYPE: Diskette, 3.50 inch

(B) COMPUTER: IBM

(C) OPERATING SYSTEM: Windows 3.1

(D) SOFTWARE: Wordperfect 6.1 (vi) CURRENT APPLICATION DATA:

(A) APPLICATION NUMBER: 08/654,737

(B) FILING DATE: 29-MAY-1996

(C) CLASSIFICATION: Unknown (viii) ATTORNEY/AGENT INFORMATION:

(A) NAME: Thomson, William E.

(B) REGISTRATION NUMBER: 20,719

(C) REFERENCE/DOCKET NUMBER: USC-002 (ix) TELECOMMUNICATION INFORMATION:

(A) TELEPHONE: (310) 788-1050

(B) TELEFAX: (310) 788-1200

(2) INFORMATION FOR SEQ ID NO: 1

(i) SEQUENCE CHARACTERISTICS:

(A) LENGTH: 317 base pairs

(B) TYPE: Nucleic Acid

(C) STRANDEDNESS : Single

(D) TOPOLOGY: Linear (ii) MOLECULE TYPE: Genomic DNA (xi) SEQUENCE DESCRIPTION: SEQ ID NO: 1

GATGGTGACC GGAGATCTGC CGCCACCATG

GGGGCGATGG CTCCGCGCAC GCTGCTCCTG

CTGCTGGCGG CCGCCCTGGC CCCGACTCAG

ACCCGCGCGG GGCCCGGCGA CTACAAGACC

ACCATCTGCG GCAAGGGCCT GAGCGCAACG

GTAACAGGGG GCCAGAAGGG GAGGGGTTCC

AGAGGCCAAC ATCAAGCTCA TTCTCTCGAG

CGGGTGTGTC ATTGTTTGGG AAAATGGCTA

GGACATCCCG ACAAGTTTG TGGGCATCAC

CTATGCTAGC CTTAAGTAGG ATCCTTGAAT

AGGTAAGTTG CTAGCCC

(2) INFORMATION FOR SEQ ID NO: 2

(i) SEQUENCE CHARACTERISTICS:

(A) LENGTH: 5865 base pairs

(B) TYPE: Nucleic Acid

(C) STRANDEDNESS: Double

(D) TOPOLOGY: Circular (ii) MOLECULE TYPE: Vector DNA

(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 2

1 TTTGAAAGAC CCCACCCGTA GGTGGCAAGC TAGCTTAAGT AACGCCACTT TGCAAGGCAT

61 GGAAAAATAC ATAACTGAGA ATAGAAAAGT TCAGATCAAG GTCAGGAACA AAGAAACAGC

121 TGAATACCAA ACAGGATATC TGTGGTAAGC GGTTCCTGCC CCGGCTCAGG GCCAAGAACA

181 GATGAGACAG CTGAGTGATG GGCCAAACAG GATATCTGTG GTAAGCAGTT CCTGCCCCGG

241 CTCGGGGCCA AGAACAGATG GTCCCCAGAT GCGGTCCAGC CCTCAGCAGT TTCTAGTGAA

301 TCATCAGATG TTTCCAGGGT GCCCCAAGGA CCTGAAAATG ACCCTGTACC TTATTTGAAC

361 TAACCAATCA GTTCGCTTCT CGCTTCTGTT CGCGCGCTTC CGCTCTCCGA GCTCAATAAA

421 AGAGCCCACA ACCCCTCACT CGGCGCGCCA GTCTTCCGAT AGACTGCGTC GCCCGGGTAC

481 CCGTATTCCC AATAAAGCCT CTTGCTGTTT GCATCCGAAT CGTGGTCTCG CTGTTCCTTG

541 GGAGGGTCTC CTCTGAGTGA TTGACTACCC ACGACGGGGG TCTTTCATTT GGGGGCTCGT

601 CCGGGATTTG GAGACCCCTG CCCAGGGACC ACCGACCCAC CACCGGGAGG TAAGCTGGCC

661 AGCAACTTAT CTGTGTCTGT CCGATTGTCT AGTGTCTATG TTTGATGTTA TGCGCCTGCG

721 TCTGTACTAG TTAGCTAACT AGCTCTGTAT CTGGCGGACC CGTGGTGGAA CTGACGAGTT

781 CTGAACACCC GGCCGCAACC CTGGGAGACG TCCCAGGGAC TTTGGGGGCC GTTTTTGTGG

841 CCCGACCTGA GGAAGGGAGT CGATGTGGAA TCCGACCCCG TCAGGATATG TGGTTCTGGT

901 AGGAGACGAG AACCTAAAAC AGTTCCCGCC TCCGTCTGAA TTTTTGCTTT CGGTTTGGAA

961 CCGAAGCCGC GCGTCTTGTC TGCTGCAGCG CTGCAGCATC GTTCTGTGTT GTCTCTGTCT

1021 GACTGTGTTT CTGTATTTGT CTGAAAATTA GGGCCAGACT GTTACCACTC CCTTAAGTTT

1081 GACCTTAGGT CACTGGAAAG ATGTCGAGCG GATCGCTCAC AACCAGTCGG TAGATGTCAA

1141 GAAGAGACGT TGGGTTACCT TCTGCTCTGC AGAATGGCCA ACCTTTAACG TCGGATGGCC 1201 GCGAGACGGC ACCTTTAACC GAGACCTCAT CACCCAGGTT AAGATCAAGG TCTTTTCACC 1261 TGGCCCGCAT GGACACCCAG ACCAGGTCCC CTACATCGTG ACCTGGGAAG CCTTGGCTTT 1321 TGACCCCCCT CCCTGGGTCA AGCCCTTTGT ACACCCTAAG CCTCCGCCTC CTCTTCCTCC

1381 ATCCGCCCCG TCTCTCCCCC TTGAACCTCC TCGTTCGACC CCGCCTCGAT CCTCCCTTTA 1441 TCCAGCCCTC ACTCCTTCTC TAGGCGCCGG AATTCGCGGC CGCTACGTAG TCGACTCGCT 1501 GTGGAATGTG TGTCAGTTAG GGTGTGGAAA GTCCCCAGGC TCCCCAGCAG GCAGAAGTAT 1561 GCAAAGCATG CATCTCAATT AGTCAGCAAC CAGGTGTGGA AAGTCCCCAG GCTCCCCAGC 1621 AGGCAGAAGT ATGCAAAGCA TGCATCTCAA TTAGTCAGCA ACCATAGTCC CGCCCCTAAC 1681 TCCGCCCATC CCGCCCCTAA CTCCGCCCAG TTCCGCCCAT TCTCCGCCCC ATGGCTGACT 1741 AATTTTTTTT ATTTATGCAG AGGCCGAGGC CGCCTCGGCC TCTGAGCTAT TCCAGAGTA 1801 GTGAGGAGGC TTTTTTGGAG GCCTAGGCTT TTGCAAAAAG CTCGAAGATC AATTCCGATC 1861 TGATCAAGAG ACAGGATGAG GATCGTTTCG CATGATTGAA CAAGATGGAT TGCACGCAGG 1921 TTCTCCGGCC GCTTGGGTGG AGAGGCTATT CGGCTATGAC TGGGCACAAC AGACAATCGG 1981 CTGCTCTGAT GCCGCCGTGT TCCGGCTGTC AGCGCAGGGG CGCCCGGTTC TTTTTGTCAA 2041 GACCGACCTG TCCGGTGCCC TGAATGAACT GCAGGACGAG GCAGCGCGGC TATCGTGGCT 2101 GGCCACGACG GGCGTTCCTT GCGCAGCTGT GCTCGACGTT GTCACTGAAG CGGGAAGGGA 2161 CTGGCTGCTA TTGGGCGAAG TGCCGGGGCA GGATCTCCTG TCATCTCACC TTGCTCCTGC 2221 CGAGAAAGTA TCCATCATGG CTGATGCAAT GCGGCGGCTG CATACGCTTG ATCCGGCTAC 2281 CTGCCCATTC GACCACCAAG CGAAACATCG CATCGAGCGA GCACGTACTC GGATGGAAGC 2341 CGGTCTTGTC GATCAGGATG ATCTGGACGA AGAGCATCAG GGGCTCGCGC CAGCCGAACT 2401 GTTCGCCAGG CTCAAGGCGC GCATGCCCGA CGGCGAGGAT CTCGTCGTGA CCCATGGCGA 2461 TGCCTGCTTG CCGAATATCA TGGTGGAAAA TGGCCGCTTT TCTGGATTCA TCGACTGTGG 2521 CCGGCTGGGT GTGGCGGACC GCTATCAGGA CATAGCGTTG GCTACCCGTG ATATTGCTGA 2581 AGAGCTTGGC GGCGAATGGG CTGACCGCTT CCTCGTGCTT TACGGTATCG CCGCTCCCGA 2641 TTCGCAGCGC ATCGCCTTCT ATCGCCTTCT TGACGAGTTC TTCTGAGCGG GACTCTGGGG 2701 TTCGTCGAGA AGCTTGGGCC CATCGATAAA ATAAAAGATT TTATTTAGTC TCCAGAAAAA 2761 GGGGGGAATG AAAGACCCCA CCTGTAGGTT TGGCAAGCTA GCTTAAGTAA CGCCATTTTG 2821 CAAGGCATGG AAAAATACAT AACTGAGAAT AGAGAAGTTC AGATCAAGGT CAGGAACAGA 2881 TGGAACAGCT GAATATGGGC CAAACAGGAT ATCTGTGGTA AGCAGTTCCT GCCCCGGCTC 2941 AGGGCCAAGA ACAGATGGAA CAGCTGAATA TGGGCCAAAC AGGATATCTG TGGTAAGCAG 3001 TTCCTGCCCC GGCTCAGGGC CAAGAACAGA TGGTCCCCAG ATGCGGTCCA GCCCTCAGCA 3061 GTTTCTAGAG AACCATCAGA TGTTTCCAGG GTGCCCCAAG GACCTGAAAT GACCCTGTGC 3121 CTTATTTGAA CTAACCAATC AGTTCGCTTC TCGCTTCTGT TCGCGCGCTT CTGCTCCCCG 3181 AGCTCAATAA AAGAGCCCAC AACCCCTCAC TCGGGGCGCC AGTCCTCCGA TTGACTGAGT 3241 CGCCCGGGTA CCCGTGTATC CAATAAACCC TCTTGCAGTT GCATCCGACT TGTGGTCTCG 3301 CTGTTCCTTG GGAGGGTCTC CTCTGAGTGA TTGACTACCC GTCAGCGGGG GTCTTTCATT 3361 TGGGGGCTCG TCCGGGATCG GGAGACCCCT GCCCAGGGAC CACCGACCCA CCACCGGGAG 3421 GTAAGCTGGC TGCCTCGCGC GTTTCGGTGA TGACGGTGAA AACCTCTGAC ACATGCAGCT 3481 CCCGGAGACG GTCACAGCTT GTCTGTAAGC GGATGCCGGG AGCAGACAAG CCCGTCAGGG 3541 CGCGTCAGCG GGTGTTGGCG GGTGTCGGGG CGCAGCCATG ACCCAGTCAC GTAGCGATAG 3601 CGGAGTGTAT ACTGGCTTAA CTATGCGGCA TCAGAGCAGA TTGTACTGAG AGTGCACCAT 3661 ATGCGGTGTG AAATACCGCA CAGATGCGTA AGGAGAAAAT ACCGCATCAG GCGCTCTTCC 3721 GCTTCCTCGC TCACTGACTC GCTGCGCTCG GTCGTTCGGC TGCGGCGAGC GGTATCAGCT 3781 CACTCAAAGG CGGTAATACG GTTATCCACA GAATCAGGGG ATAACGCAGG AAAGAACATG 3841 TGAGCAAAAG GCCAGCAAAA GGCCAGGAAC CGTAAAAAGG CCGCGTTGCT GGCGTTTTTC

3901 CATAGGCTCC GCCCCCCTGA CGAGCATCAC AAAAATCGAC GCTCAAGTCA GAGGTGGCGA

3961 AACCCGACAG GACTATAAAG ATACCAGGCG TTTCCCCCTG GAAGCTCCCT CGTGCGCTCT

4021 CCTGTTCCGA CCCTGCCGCT TACCGGATAC CTGTCCGCCT TTCTCCCTTC GGGAAGCGTG 4081 GCGCTTTCTC AATGCTCACG CTGTAGGTAT CTCAGTTCGG TGTAGGTCGT TCGCTCCAAG 4141 CTGGGCTGTG TGCACGAACC CCCCGTTCAG CCCGACCGCT GCGCCTTATC CGGTAACTAT 4201 CGTCTTGAGT CCAACCCGGT AAGACACGAC TTATCGCCAC TGGCAGCAGC CACTGGTAAC 4261 AGGATTAGCA GAGCGAGGTA TGTAGGCGGT GCTACAGAGT TCTTGAAGTG GTGGCCTAAC 4321 TACGGCTACA CTAGAAGGAC AGTATTTGGT ATCTGCGCTC TGCTGAAGCC AGTTACCTTC 4381 GGAAAAAGAG TTGGTAGCTC TTGATCCGGC AAACAAACCA CCGCTGGTAG CGGTGGTTTT 4441 TTTGTTTGCA AGCAGCAGAT TACGCGCAGA AAAAAAGGAT CTCAAGAAGA TCCTTTGATC 4501 TTTTCTACGG GGTCTGACGC TCAGTGGAAC GAAAACTCAC GTTAAGGGAT TTTGGTCATG 4561 AGATTATCAA AAAGGATCTT CACCTAGATC CTTTTAAATT AAAAATGAAG TTTTAAATCA 4621 ATCTAAAGTA TATATGAGTA AACTTGGTCT GACAGTTACC AATGCTTAAT CAGTGAGGCA 4681 CCTATCTCAG CGATCTGTCT ATTTCGTTCA TCCATAGTTG CCTGACTCCC CGTCGTGTAG 4741 ATAACTACGA TACGGGAGGG CTTACCATCT GGCCCCAGTG CTGCAATGAT ACCGCGAGAC 4801 CCACGCTCAC CGGCTCCAGA TTTATCAGCA ATAAACCAGC CAGCCGGAAG GGCCGAGCGC 4861 AGAAGTGGTC CTGCAACTTT ATCCGCCTCC ATCCAGTCTA TTAATTGTTG CCGGGAAGCT 4921 AGAGTAAGTA GTTCGCCAGT TAATAGTTTG CGCAACGTTG TTGCCATTGC TGCAGGCATC 4981 GTGGTGTCAC GCTCGTCGTT TGGTATGGCT TCATTCAGCT CCGGTTCCCA ACGATCAAGG 5041 CGAGTTACAT GATCCCCCAT GTTGTGCAAA AAAGCGGTTA GCTCCTTCGG TCCTCCGATC 5101 GTTGTCAGAA GTAAGTTGGC CGCAGTGTTA TCACTCATGG TTATGGCAGC ACTGCATAAT 5161 TCTCTTACTG TCATGCCATC CGTAAGATGC TTTTCTGTGA CTGGTGAGTA CTCAACCAAG 5221 TCATTCTGAG AATAGTGTAT GCGGCGACCG AGTTGCTCTT GCCCGGCGTC AACACGGGAT 5281 AATACCGCGC CACATAGCAG AACTTTAAAA GTGCTCATCA TTGGAAAACG TTCTTCGGGG 5341 CGAAAACTCT CAAGGATCTT ACCGCTGTTG AGATCCAGTT CGATGTAACC CACTCGTGCA 5401 CCCAACTGAT CTTCAGCATC TTTTACTTTC ACCAGCGTTT CTGGGTGAGC AAAAACAGGA 5461 AGGCAAAATG CCGCAAAAAA GGGAATAAGG GCGACACGGA AATGTTGAAT ACTCATACTC 5521 TTCCTTTTTC AATATTATTG AAGCATTTAT CAGGGTTATT GTCTCATGAG CGGATACATA 5581 TTTGAATGTA TTTAGAAAAA TAAACAAATA GGGGTTCCGC GCACATTTCC CCGAAAAGTG 5641 CCACCTGACG TCTAAGAAAC CATTATTATC ATGACATTAA CCTATAAAAA TAGGCGTATC 5701 ACGAGGCCCT TTCGTCTTCA AGAATTCATA CCAGATCACC GAAAACTGTC CTCCAAATGT 5761 GTCCCCCTCA CACTCCCAAA TTCGCGGGCT TCTGCCTCTT AGACCACTCT ACCCTATTCC 5821 CCACACTCAC CGGAGCCAAA GCCGCGGCCC TTCCGTTTCT TTGCT

Claims

What is claimed is:

1. A method of treating a patient for a T-cell mediated autoimmune disease

comprising:

introducing DNA comprising a sequence encoding one or more antigenic proteins

into the cells of said patient, said cells expressing in said patient a therapeutically

effective amount of said antigenic protein or proteins to restore T-cell tolerance

to said patient.

2. The process of claim 1 wherein said patient is human.

3. The process of claim 2 wherein said cells are fibrobiast cells.

4. The process of claim 3 wherein said fibrobiast cells are histocompatible.

5. The process of claim 2 wherein said DNA encodes an amino acid sequence

derived from a nervous system protein.

6. The process of claim 2 wherein the disease is multiple sclerosis, rheumatoid

arthritis, systemic lupus erythematosus, psoriasis, juvenile onset diabetes,

Sjogren's disease, thyroid disease, myasthenia gravis, or chronic inflammatory

demyelinating polyneuropathy (CIDP).

7. The method of claim 1 wherein the disease is multiple sclerosis.

8. A method of treating a human for a T-cell mediated auto immune disease

comprising:

introducing DNA comprising a sequence encoding one or more amino acid

sequence derived from a self-antigenic protein into the cells of said human, said

cells expressing in said human a therapeutical ly effective amount of said self-

antigenic protein or proteins to restore T-cell tolerance to said human.

9. A method of treating a human for multiple sclerosis comprising:

introducing DNA comprising a sequence encoding one or more amino acid

sequence derived from a nervous system protein into the cells of said human, said

cells secreting in said human a therapeutically effective amount of said self-

antigenic protein or proteins to restore T-cell tolerance to said human.

10. A method of treating a patient for a T-cell mediated autoimmune disease

comprising:

introducing mammalian cells into a patient, said cells having been treated in vitro

to insert therein a DNA segment encoding one or more antigenic protein, said

mammalian cells expressing in vivo in said patient a therapeutically effective

amount of said antigenic protein or proteins to restore T-cell tolerance to said

patient.

1 1. The process of claim 10 wherein said patient is human.

12. The process of claim 1 1 wherein said cells are fibrobiast cells.

13. The process of claim 12 wherein said fibrobiast cells are histocompatible.

14. The process of claim 11 wherein said disease is multiple sclerosis, rheumatoid

arthritis, systemic lupus erythematosus, psoriasis, juvenile onset diabetes,

Sjogren's disease, thyroid disease, or myasthenia gravis or chronic inflammatory

demyelinating polyneuropathy (CIDP).

15. The process of claim 10 wherein said disease is multiple sclerosis.

16. The process of claim 10 wherein said DNA segment has been inserted into said

cells in vitro by a recombinant vector.

17. The process of claim 10 wherein said DNA segment has been inserted into said

cells in vitro by a viral vector.

18. The process of claim 17 wherein said viral vector is a retroviral vector.

19. The process of claim 10 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system self-antigenic

protein.

20. The process of claim 1 1 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system self-antigenic

protein.

21. The process of claim 14 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a self-antigenic protein.

22. The process of claim 12 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein.

23. The process of claim 13 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein.

24. The process of claim 15 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein.

25. The process of claim 16 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein. 25. The process of claim 17 wherein the DNA segment encodes a protein comprising

an amino acid sequence derived from a nervous system protein.

26. The process of claim 18 wherein the DNA segment encodes a protein comprising

an amino acid sequence derived from a nervous system protein.

28. The process of claim 10 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

selected from the group consisting of myelin basic protein, proteolipid protein,

and myelin-oligodendrocyte glycoprotein.

29. The process of claim 1 1 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

and myelin-oligodendrocyte glycoprotein.

30. The process of claim 12 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

and myelin-oligodendrocyte glycoprotein.

31. The process of claim 13 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein selected from the group consisting of myelin basic protein, proteolipid protein,

and myelin-oligodendrocyte glycoprotein.

32. The process of claim 15 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

and myelin-oligodendrocyte glycoprotein.

33. The process of claim 16 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

selected from the group consisting of myelin basic protein, proteolipid protein, and myelin-oligodendrocyte glycoprotein.

34. The process of claim 17 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

and myelin-oligodendrocyte glycoprotein.

35. The process of claim 18 wherein said DNA segment encodes a protein

comprising an amino acid sequence derived from a nervous system protein

and myelin-oligodendrocyte glycoprotein.

36. The process of claim 10 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

37. The process of claim 1 1 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

38. The process of claim 12 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

39. The process of claim 13 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

40. The process of claim 15 wherein said DNA segment encodes an protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

41. The process of claim 16 wherein said DNA segment encodes an protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

42. The process of claim 17 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

43. The process of claim 18 wherein said DNA segment encodes a protein

comprising an encephalitogenic epitope selected from the group consisting of

encephalitogenic epitopes of myelin basic protein, encephalitogenic epitopes of

myelin-oligodendrocyte glycoprotein, and encephalitogenic epitopes of

proteolipid protein.

44. The process of any one of claims 19-43 wherein said DNA segment additionally

comprises a hydrophobic leader sequence, said hydrophobic leader sequence

enabling the gene product to be synthesized in an endoplasmic reticulum for later

constitutive secretion.

45. The process of any one of claims 19-43 wherein said DNA segment further

comprises a Kozak box, said Kozak box permitting efficient translation of an

mRNA transcribed from said DNA segment.

46. The process of any one of claims 19-43 wherein said DNA segment further

comprises a codon corresponding to a charged amino acid at the 3' end to ensure

that the protein is not retained in membrane.

47. The process of any one of claims 19-43 wherein said DNA segment further

comprises one or more restriction sites to permit insertion of additional gene

sequences.

48. The process of any one of claims 19-43 wherein said DNA sequence encodes

amino acids 101-157 of proteolipid protein.

49. A method of treating a human patient for multiple sclerosis comprising:

introducing mammalian cells into said human patient, said mammalian cells

having been treated in vitro to insert therein a DNA segment encoding one or more encephalitogenic epitope derived from nervous system protein, said

mammalian cells expressing in vivo in said human patient a therapeutically

effective amount of said encephalitogenic epitope or epitopes to restore T-cell

tolerance to said human patient.

50. The method of claim 49 wherein said mammalian cells are fibroblasts cells.

51. The method of claim 50 wherein said mammalian fibrobiast cells are

histocompatible.

52. A method of treating a human patient for multiple sclerosis comprising:

introducing histocompatible fibrobiast cells into said human patient, said

histocompatible fibrobiast cells having been treated in vitro to insert therein a

DNA segment encoding amino acids 101-157 of proteolipid protein, said DNA

segment introduced into said histocompatible fibroblasts cells in vitro by a

recombinant retroviral vector, said DNA sequence comprising a hydrophobic

leader sequence whereby said leader sequence enables said amino acids 101 -157

of proteolipid protein to be synthesized in the endoplasmic reticulum of said

histocompatible fibrobiast cells for later constitutive secretion, said DNA

segment further comprising a Kozak box permitting efficient translation of

mRNA transcribed from said DNA segment, said DNA segment further

comprising a codon corresponding to a charged amino acid at the 3' end to ensure

that the protein is not retained in membrane, said DNA segment further comprising one or more restriction sites to permit insertion of additional gene

sequences, whereby the gene product or gene products of said DNA segment is

expressed in said human in a therapeutically effective amount to restore T-cell

tolerance to said human.

53. An engineered cell comprising a gene encoding one or more antigenic protein

which can be expressed, wherein said gene has been introduced into the cell by

means of a recombinant vector.

54. An engineered cell comprising a gene encoding one or more antigenic protein

which can be secreted, wherein said gene has been introduced into the cell by

means of a recombinant vector.

55. An engineered cell comprising a gene encoding one or more encephalitogenic

epitope which can be expressed, wherein said gene has been introduced into the

cell by means of a recombinant vector.

56. An engineered cell comprising a gene encoding one or more encephalitogenic

epitope which can be secreted, wherein said gene has been introduced into the

cell by means of a recombinant vector.

57. Any one of claims 53-56 wherein said recombinant vector is a retroviral vector.

58. The cell of claim 56 wherein said gene comprises the sequence encoding amino

acids 101-157 of proteolipid protein.