Patent Publication Number: US-5530178-A

Title: Mutant mouse lacking CD8 surface marker

Description:
This application is a continuation-in-part of application Ser. No. 07/707,036, filed May 29, 1991, now abandoned. 
    
    
     The invention is a mutant mouse lacking the CD8 surface marker on its T lymphocytes. The invention as expressed, for example, in mutant mice is useful for the study of CD8 in T cell maturation and the function of CD8 +   T cells in the immune system. The invention is useful in the development of clinical or diagnostic applications relating to auto-immune diseases, viral infections, parasite infections and other such medical conditions as will be apparent to the skilled person. 
     T cells recognize processed antigenic peptides in association with class I or class II molecules encoded by the major histocompatibility complex (MHC). The antigen specificity of T cells is mainly attributed to the T cell receptor (TcR). Class I and class II MHC restricted T cells can be distinguished from each other by the presence of the surface markers CD8 and CD4, respectively. CD8 +   T cells are usually cytotoxic cells (CTL) responding to antigenic challenge by lysis of the target cells, while CD4 +   T cells are helper cells which produce lymphokines and play a role in the activation or proliferation or both of B cells, CTL, and macrophages. 
     Maturation of T cells in the thymus involves the processes of selection for tolerance of self-antigens (negative selection) and acquisition of restriction to self-MHC molecules (positive selection). T cell precursors entering the thymus initially do not express CD4, CD8 or CD3 on their surface. They differentiate in the thymus through a series of intermediates, including a transient stage of CD8 +   cells which lack T cell receptor, to a stage when CD4, CD8, and low levels of TcR are expressed on the cell surface. It is at this stage of development that the T cells undergo positive and negative selection and eventually emerge from the thymus as mature CD8 +  CD4 -   or CD4 +  CD8 -   (single positive) T cells. 
     The present invention provides a mutant mouse lacking the CD8 surface marker on its T cells. Particularly described are genetically manipulated mice that lack cell surface expression of CD8. The invention was obtained in mice by disruption of the coding sequence of the murine Lyt-2 gene by homologous recombination (Smithies et al., 1985) in embryonic stem (ES) cells (Thomas and Capecchi, 1987). The ES cells have the potential to contribute to all tissues including the germ-line when they are introduced into mouse preimplantation embryos (Gossler et al., 1986; Robertson et al., 1986). Subsequent breeding of the mice allows the generation of a new mouse strain, homozygous for the genetic change. 
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS 
     FIG. 1 shows schematic diagrams of the mouse Lyt-2 gene and the Lyt-2 construct for homologous recombination. The boxes indicate exons of the Lyt-2 gene with black shading to denote coding regions. The neomycin resistant gene (neo) was inserted as described in Experimental Procedures. Arrows indicate the positions and directions (5&#39; to 3&#39;) of the primers used in PCR screening as described in Experimental Procedures. Restriction enzyme sites are B, BamHI; E, EcoRI; H, HindIII. 
     FIGS. 2A, 2B, 2C, 2G, 2H, 2I, 2M, 2N, and 2O show flow cytometric analyses of thymus cells from wild-type mice (+/+) and mice heterozygous (+/-) and homozygous (-/-) for the disrupted Lyt-2 gene. FIGS. 2D, 2E, 2F, 2J, 2K, 2L, 2P, 2Q, and 2R show flow cytometric analyses of lymph node cells from wild-type mice (+/+) and mice heterozygous (+/-) and homozygous (-/-) for the disrupted Lyt-2 gene. Samples were stained for Lyt-2 and CD4 (FIGS. 2A, 2B, 2C, 2D, 2E, and 2F), Lyt-3 and CD4 (FIGS. 2G, 2H, 2I, 2J, 2K, and 2L), or CD3 and CD4 (FIGS. 2M, 2N, 2O, 2P, 2Q, and 2R). 
     FIG. 3 shows cytotoxic activities of T cells from spleens of wild-type mice (+/+), heterozygous (+/-) and homozygous (-/-) mutant mice. (A) Cytotoxic activities against alloantigens. Effector cells (H-2 b/d ) were stimulated in vitro with irradiated allogeneic spleen cells from SWR (H-2 1 ) mouse strain as described in Experimental Procedures. Target cells were concanavalin A induced lymphoblasts from SWR and C57BL/6 (H-2 b ) mice. (B) Anti-viral cytotoxic activities. Effector cells were from mice (H-2b) primed in vivo with vaccinia virus as described in Experimental Procedures. Target cells were YAC cells and MC57 cells either uninfected or infected with vaccinia virus. 
     FIG. 4 shows proliferation of T cells from spleens of wild-type mice (+/+), heterozygous (+/-) and homozygous (-/-) mutant mice (H-2b) in response to allogeneic spleen cells from SWR (H-2 q ), B10.BR (H-2 k ), B6 bm12 (H-2 bm  12), and B6 bm1 (H-2 bm1 ) mouse strains. Spleen cells from the same animal (SYN) and from C57BL/6 (H-2 b ) mice were used as controls. 
    
    
     Generation of Mice Without CD8 Surface Expression 
     CD8 in the mouse is encoded by two genes, Lyt-2 and Lyt-3 (Zamoyska et al., 1985; Nakauchi et al., 1987) and is expressed on the T cell surface predominantly as a disulfide-linked heterodimer of Lyt-2 and Lyt-3 (Ledbetter et al., 1981; Walker et al., 1984a; b). Lyt-2 can also be expressed on the cell surface as a homodimer in transfected cells (Zamoyska et al., 1985; Gorman et al., 1988), but the surface expression of Lyt-3, at least in T cell lines, appears to require the presence of the Lyt-2 molecule (Blanc et al., 1988; Gorman et al., 1988; Schmidt-Ullrich and Eichmann, 1990). Therefore, the Lyt-2 gene was disrupted to generate a mutant mouse strain without cell surface expression of CD8. The Lyt-2 gene contains five exons spanning a region of 4.4 kb (Liaw et al., 1986). To disrupt the Lyt-2 gene by homologous recombination, a 2.2 kb HindIII-BamHI DNA fragment containing exons 1, 2, and 3 of the Lyt-2 gene was used as a construct and the coding sequence was interrupted by inserting the neomycin resistance gene (Thomas and Capecchi, 1987) into the EcoRI site of exon 1 (FIG. 1). This DNA construct was introduced into D3 embryonic stem cells (Doetschman et al., 1985) by electroporation. G418-resistant colonies were screened for the homologous recombination event between the construct and the endogenous Lyt-2 gene by the polymerase chain reaction (PCR). The average frequency of homologous recombination was about 1 in 10 7  electroporated cells or 1 in 200 G418-resistant clones. 
     ES cell lines with the disrupted Lyt-2 gene were injected into 3.5 day old C57BL/6 blastocysts and chimeric mice were obtained. Male chimeric mice were tested for germ-line transmission of the mutation and chimeric mice from one of the cell lines were shown to generate offspring heterozygous for the mutation. Mice carrying the disrupted Lyt-2 gene were identified by tail DNA analysis and were interbred to obtain mice homozygous for the mutant gene. 
     Phenotypic Analysis of Mutant Mice 
     Mice heterozygous and homozygous for the disrupted Lyt-2 gene appeared to be healthy and were fertile. Gross inspection of the lymphoid organs of the homozygous mice (i.e. thymus, lymph node, spleen) did not show any sign of atrophy. The anatomical distribution of lymphoid and stromal cells in the thymus of the mutant mice was shown to be normal by immunohistochemical methods using monoclonal antibodies against CD3, CD4 and Lyt-2 on thymocytes, and antibodies ER-TR4 and ER-TR5 which recognize cortical and medullary epithelial cells, respectively (data not shown). Numbers of cells in lymphoid organs were similar to those of normal mice. The ratio of T and B cells in lymph nodes of these mice was normal as identified by antibodies specified for Thy-1.2  and immunoglobulin M, respectively, in flow cytometric analysis (data not shown). Both the heterozygous and homozygous mice expressed normal levels of MHC class I and class II proteins as determined by florescence cell activating staining (data not shown). &#34;Normal&#34; here refers to that expression level found in wild-type mice. 
     Surface expression of Lyt-2 was not detected on thymocytes and lymph node cells from mice homozygous for the disrupted Lyt-2 gene (FIG. 2A). Interestingly, the intensity of the staining for Lyt-2 in heterozygous mice was about half of that of wild-type mice. These data suggest that the Lyt-2 genes of both maternal and paternal origin contribute to the level of Lyt-2 expression. Similar results were found when these cells were stained with a monoclonal antibody against Lyt-3 (FIG. 2B), suggesting that surface expression of Lyt-3 is dependent on concomitant Lyt-2 expression in most, if not all, thymocytes and T lymphocytes. The reduction in the level of Lyt-3 surface expression in heterozygous mice suggests that Lyt-2 is the limiting molecule for surface expression of CD8. 
     Absence of Class I MHC Restricted Cytotoxic T Cells 
     Murine cytotoxic T cells are usually of the CD8 +  CD4 -   phenotype. This population was absent from the thymus and lymph nodes of mice homozygous for the disrupted Lyt-2 gene (FIG. 2A and B). It is possible that mature T cells, normally bearing CD8, might still be present in the homozygous mouse but would now simply be lacking CD8 expression on the cell surface. The thymocytes and lymph node cells were therefore stained with antibodies against CD4 and CD3 to examine this possibility (FIG. 2C). There is no indication of a significant CD3 +  CD4 -   population. 
     CD8 +   T cells in mice have cytotoxic effector functions. To address the question whether peripheral T cells from mice without CD8 expression could mount a cytotoxic response against alloantigens, spleen cells of these mice (H-2 b/d ) were stimulated with allogeneic cells (H-2 q ). The cytotoxic activity of the responder cells after five days of stimulation was assessed in a standard  51  Cr release assay (FIG. 3A). T cells from heterozygous mice, which have a decreased level of CD8 expression, generated a cytotoxic response against H-2 q  alloantigens which was comparable to the response of T cells from wild-type mice. The homozygous mice lacking CD8 +   T cells, however, did not develop a significant cytolytic T cell response against the specific target cells. 
     Mice infected with vaccinia virus mount a specific cytotoxic T cell response against the virus. The anti-viral cytotoxic function of T cells in mice primed in vivo with vaccinia infection was studied (FIG. 3B). Spleen cells from wild-type mice and mice heterozygous for the disrupted Lyt-2 gene lysed vaccinia infected MC57 cells but the lysis of uninfected MC57 cells or YAC cells was insignificant. The CD8 defective mice did not display a specific anti-vaccinia cytolytic activity although some nonspecific cytotoxicity was detected. 
     Although class I MHC restricted cytotoxic activity against alloantigens and viral antigens was not detected in bulk cultures, the possibility that very low numbers of cytotoxic T cells may be present in these mice has not yet been completely excluded. 
     Presence of CD4 +   Helper T Cells 
     Intrathymic maturation of helper T cells in mice defective in CD8 expression was studied by staining thymocytes with monoclonal antibodies specific for CD4 and other T Cell surface proteins. The sizes of thymocyte subsets identified by CD4 and CD8 (Lyt-2 and Lyt-3) surface expression appeared normal in Lyt-2  defective heterozygous mice despite lower levels of Lyt-2 and Lyt-3 expression (FIG. 2A and B). In homozygous mice, the CD4 -  CD8 -   (double negative) population appears to be unchanged, but the population that would correspond to the CD4 +  CD8 +  (double positive) stage seems to have merged with the CD4 +  CD8 -  subpopulation. 
     Thymus and lymph node cells were examined by staining with monoclonal antibodies against CD4 and CD3 to study if the lack of surface expression of CD8 (Lyt-2 and Lyt-3) would affect the maturation of CD4 +   T lymphocytes. Thymocytes can be divided into three subpopulations (CD3 - , CD3 low  and CD3 high ) with the level of CD3 expression corresponding to the degree of differentiation. Thymuses from homozygous mice contained immature T cells at the different stages of development and the ratio of the subpopulations was similar to that found in heterozygous and wild-type mice (FIG. 2C). These findings suggest that in the absence of surface Lyt-2 expression the process of thymic maturation and selection of CD4 +   T cells is relatively normal. 
     The proliferative potential of T cells from CD8 defective mice against alloantigens was studied. Spleen cells from these mice (H-2 b ) were stimulated with allogeneic cells disparate in class I MHC (H-2 bm1 ), class II MHC (H-2 bm  12) or both (H-2 q  and H-2 k ). The responses in proliferation against complete H-2 differences and a class II MHC difference seemed to be similar among the three types of mice (FIG. 4) and interleukin-2 (IL-2) secretion was detected in these responses (data not shown). However, homozygous mice showed a decreased response against a class I MHC difference while the response of heterozygous mice was comparable to the response of wild-type mice. These data suggest that, although the CD8 +   T cells which recognize allogeneic class I MHC molecules were not detected in homozygous mice, CD4 +   T cells are functional and can respond to class II MHC alloantigens. 
     The in vivo anti-viral humoral response in mice defective in CD8 expression was studied by injecting mice with vesicular stomatitis virus (VSV). The efficiency of the humoral response was assessed by measuring levels of immunoglobulin M (IgM) and immunoglobulin G (IgG) virus neutralizing antibodies (Table 1). An early onset of anti-VSV IgM was detected on day 4 after viral infection. This was replaced by anti-VSV IgG by day 8 and the levels of IgG were still maintained on day 16 after infection. The levels of anti-VSV neutralizing IgM and IgG antibodies and their kinetics of induction were comparable among the wild-type mice and mice with the disrupted Lyt-2 genes. Since the switch from IgM to IgG is strictly dependent on helper T cells (Gupta et al., 1986), these results confirm that CD4 +   helper T cells do provide help to B cells in mice defective in CD8 expression. 
     The present invention has enabled a showing that the absence of CD8 expression in the mutant mice prevents the development of class I MHC restricted cytotoxic T cells. Recognition of the appropriate class I MHC molecule by T cell receptor has been shown to be a decisive interaction for positive selection of cytotoxic T cells (Kisielow et al., 1988; Sha et al., 1988; Pircher et al., 1989). The data derived pursuant to the invention shows that the presence of CD8 is also necessary for the development of functional class I MHC restricted T cells. While the T cell receptor appears to recognize the polymorphic domains of the class I MHC molecule, CD8 most likely interacts with the monomorphic alpha-3 domain of class I MHC (Connolly et al., 1988; Salter et al., 1990). The lack of either one of these interactions results in the block of the development of cytotoxic T cells. The cytoplasmic portion of CD8 has been shown to be associated with a protein tyrosine kinase P56 lck  (Veillette et al., 1988; Barber et al., 1989; Rudd et al., 1989; Shaw et al, 1990; Turner et al., 1990) and could thus be involved in signal transduction during T cell ontogeny (Nakayama et al., 1989; Veillette et al., 1989). The importance of the cytoplasmic tail of CD8 could be studied by using the mice of the invention as recipients of transgenes carrying specific mutations of the CD8 gene. 
     In contrast to the lack of mature cytotoxic T cells, the maturation of class II MHC restricted helper T cells appears to be unaffected by the absence of CD8 surface expression. Hence, surface expression of CD8 on the early CD8 +  CD4 -  TcR -   population, as well as on the more mature CD4 +  CD8 +  TcR low  thymocyte population, is not obligatory for the differentiation of CD4 +   T lymphocytes. The proliferative response against class II MHC alloantigens and the helper T cell dependent B cell response following infection with VSV are normal in homozygous mice. These results indicate that CD4 +   T cells are functional in the mutant mice. 
     The mutant mouse strain provides a model of an immune system that specifically lacks the CD8 +   T cell population. Therefore, these mice should be valuable to study the involvement of CD8 +   T cells in infections, in the pathogenesis of autoimmune diseases and in the rejection of tumor or tissue transplants. 
     
                       TABLE 1                                                     
______________________________________                                    
Neutralizing anti-VSV response in mice defective                          
in CD8 expression                                                         
        Titers of neutralizing activities.sup.a &#39;                         
        (log.sub.2 × 10.sup.-1) in sera from mice                   
        after i.v. infection with VSV (2 × 10.sup.6 PFU)            
mouse strain                                                              
          day 4      day 8     day 12  day 16                             
(CD8 genotype)                                                            
          IgM     IgG    IgM  IgG  IgM  IgG  IgG                          
______________________________________                                    
+/+       9       &lt;1     1    8    2    10   11                           
          10      &lt;1     1    8    &lt;1   11   10                           
          10      &lt;1     &lt;1   8    &lt;1   10   10                           
          10      &lt;1     &lt;1   8    --.sup.b &#39;                             
                                        --   --                           
+/-       10      &lt;1     1    8    &lt;1   11   10                           
          9       &lt;1     2    8    &lt;1   10   10                           
          9       &lt;1     1    11   &lt;1   12   12                           
          10      &lt;1     --   --   --   --   --                           
-/-       8       &lt;1     1    7    1     9    8                           
          9       &lt;1     2    6    1     9    8                           
          9       &lt;1     &lt;1   9    &lt;1   12   11                           
          9       &lt;1     1    8    &lt;1   12   12                           
______________________________________                                    
 .sup.a &#39; Neutralizing IgM and IgG titers were determined as described in 
 Experimental Procedures. Titers represent twofold dilution steps of sera 
 starting with 1:40.                                                      
 .sup.b &#39; Not determined because mice had died.                           
 
    
     EXPERIMENTAL PROCEDURES 
     Production of Mutant Mice Lacking CD8 Expression 
     The 2.2 kb HindIII-BamHI DNA fragment containing exon 1 to exon 3 of the Lyt-2 gene was used as a construct for homologous recombination. The 1.2 kb blunt-ended XhoI-BamHI fragment of the plasmid pMC1polA, which contains the neomycin resistant gene (Thomas and Capecchi, 1987), was inserted in opposite transcriptional orientation into the blunt-ended EcoRI site in the first exon of the Lyt-2 gene construct. 
     D3 embryonic stem cells from 129/J mice were maintained in the undifferentiated state either by growth on a feeder layer of mitomycin-C treated primary embryonic fibroblasts (Doetschman et al., 1985) or in culture medium supplemented with leukemia inhibitory factor (Smith et al., 1988). 
     Electroporation of embryonic stem cells, selection of G418-resistant colonies and polymerase chain reaction (PCR) screening for homologous recombination were carried out as described (Joyner et al., 1989). A primer specific for the neomycin resistance gene in the construct (5&#39;-AACGCACGGGTGTTGGGTCGTTTG-3&#39;) (SEQ. ID NO. 1) , and another primer specific for the Lyt-2 gene upstream of the construct (5&#39;-ATTCAAGGCCAACCTTTGCC-3&#39;) (SEQ. ID NO. 2) were used in PCR. Homologous recombination was subsequently confirmed by genomic Southern blot hybridization. Chimeric mice were produced by injection of the embryonic stem cells into 3.5 day old blastocysts as described (Bradley, 1987). The contribution of embryonic stem cells to the germ-line of chimeric mice was assessed by breeding with (C57BL/6×DBA/2)F1 females and screening for agouti offspring. Germ-line transmission of the Lyt-2 mutation was confirmed by Southern analysis of the tail DNA and mice heterozygous for the mutant gene were interbred to homozygosity. 
     Flow Cytometric Analysis 
     Single cell suspensions from thymus and lymph nodes of 6-8 week old mice were made and 5×10 5  cells were stained with monoclonal antibodies for 30 minutes at 4° C. in 100 μl phosphate buffer saline containing 1% BSA and 0.1% sodium azide. Cells were then washed and analysed for single and double-colour flow cytometric analysis on a FACScan (Becton Dickinson, Inc.). Monoclonal antibodies used were: Lyt-2 (53-6.7, Becton Dickinson, Inc.), Lyt-3 (53-5.8, PharMingen, Inc.), L3T4 (GK1.5, Becton Dickinson Inc.), CD3 (145-2C11, PharMingen, Inc.), thy-1.2 (30-H12, Becton Dickinson, Inc.), and goat anti-mouse immunoglobulin G (Southern Biotechnology Associates, Inc.). 
     Cytotoxicity Assay 
     Cytotoxic assays were performed as described (Schilham et al., 1986). Alloreactive cytotoxic T lymphocytes were generated in a 5 day mixed lymphocyte culture. Responder spleen cells (2×10 6  /ml) were from adult (6-8 weeks) mice with normal, functional Lyt-2 gene (+/+), and mice heterozygous (+/-) and homozygous (-/-) for the disrupted Lyt-2 gene. These mice were of haplotype H-2 b/d . Stimulators were irradiated spleen cells (5×10 6  /ml, 3000 rad) from SWR (H-2 q ) and C57BL/6 (H-2 b ) mice. Target cells were lymphoblasts induced by concanavalin A (2.5 μg/ml) for three days and labelled with  51  chromium (Amersham). 
     Cytotoxic T cells specific for viral antigens were generated as follows: mice were primed in vivo by intravenous injection of vaccinia-WR (2×10 6  plaque forming unit (PFU)/mouse) 6 days prior to preparation of spleen cells. Target cells were MC57 fibroblasts infected with vaccinia-WR (5 PFU/cell) at the time of  51  Cr labelling. Uninfected MC57 cells and YAC cells were used as controls for nonspecific cytotoxic activity. 
     The  51  chromium release assay was performed by incubating 1×10 4  labeled target cells with different numbers of responder cells in a 0.2 ml culture medium in round-bottom microtiter plates. Plates were spun at 400 g for 5 minutes and then incubated for 4 hours at 37° C. After incubation, aliquots of supernatant were collected for determination of radioactivity in a γ-counter (LKB, Inc.) Percent specific lysis was calculated from cpm as 100×(experimental-spontaneous)/(total-spontaneous), whereas spontaneous release was determined in the absence of responder cells and total release was determined in the presence of 1N acetic acid. Each responder/target cell ratio was tested in duplicate. 
     Proliferation Assay 
     Responder cells were spleen cells from adult (6-8 weeks) mice with functional Lyt-2 gene and mice heterozygous and homozygous for the disrupted Lyt-2 gene. These mice were of haplotype H-2 b . Stimulator cells were irradiated (3000 R) spleen cells from the same mouse as the responder cells (syngeneic), and from mouse strains C57BL/6 (H-2 b ), SWR(H-2 q ), C57BL/6 bml (H- bml ) or C57BL/6 bml2 (H-2 bml2 ). 5×10 5  Responder cells were cultured with 5×10 5  stimulator cells in a 0.2 ml culture medium for 3 days and  3  H-thymidine uptake by cells after 16 hours incubation was determined in triplicates. The data represent the mean of triplicate determinations. 
     Neutralizing Antibody Determinations 
     Vesicular Stomatitis virus (Indiana strain) was injected intravenously (2×10 6  PFU/mouse) into 6-8 week old wild-type mice and mice heterozygous and homozygous for the disrupted Lyt-2 gene. Four mice were used per group. Blood samples were collected on day 4, 8, 12 and 16 after infection. A virus neutralization assay was performed as previously described (Roost et al., 1988). The neutralizing antibody titer was defined as the highest dilution of serum that reduced the number of plaques to half of the control. The titer of IgG was determined after reduction of IgM by pre-treatment of sera with 0.1M B-mercaptoethanol in saline for 1 hour at room temperature (Scott and Gershon, 1970) before the assay. Titers of sera without β-mercaptoethanol treatment were taken as the total titers of both IgG and IgM. 
     Deposits 
     ES cell line with the disrupted Lyt-2 gene as shown in FIG. 1 has been deposited in the American Type Culture Collection, Rockville, Md., and given ATCC Accession No. CRL 11116. 
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SEQUENCE LISTING                                                          
(1) GENERAL INFORMATION:                                                  
(iii) NUMBER OF SEQUENCES: 2                                              
(2) INFORMATION FOR SEQ ID NO:1:                                          
(i) SEQUENCE CHARACTERISTICS:                                             
(A) LENGTH: 24 base pairs                                                 
(B) TYPE: nucleic acid                                                    
(C) STRANDEDNESS: single                                                  
(D) TOPOLOGY: linear                                                      
(ii) MOLECULE TYPE: DNA                                                   
(xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:                                   
AACGCACGGGTGTTGGGTCGTTTG24                                                
(2) INFORMATION FOR SEQ ID NO:2:                                          
(i) SEQUENCE CHARACTERISTICS:                                             
(A) LENGTH: 20 base pairs                                                 
(B) TYPE: nucleic acid                                                    
(C) STRANDEDNESS: single                                                  
(D) TOPOLOGY: linear                                                      
(ii) MOLECULE TYPE: DNA                                                   
 (xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:                                  
ATTCAAGGCCAACCTTTGCC20                                                    
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