T cell-mediated immunotherapy is an attractive strategy for treatment in various disease areas. In this therapeutic approach, the CD3 complex is one of the key molecules to modulate T cell functions; however, in many cases, we cannot evaluate the drug candidates in animal experiments because the therapeutics, usually monoclonal antibodies specific to human CD3, cannot react to mouse endogenous Cd3. Although immunodeficient mice transfused with human hematopoietic stem or precursor cells, known as humanized mice, are available for these studies, mice humanized in this manner are not completely immune competent. In this study we have succeeded in establishing a novel mouse strain in which all the three components of the Cd3 complex - Cd3ε, Cd3δ, and Cd3γ - are replaced by their human counterparts, CD3E, CD3D, and CD3G. Basic immunological assessments have confirmed that this strain of human CD3 EDG-replaced mice are entirely immune competent, and we have also demonstrated that a bispecific antibody that simultaneously binds to human CD3 and a tumor-associated antigen (e.g. ERBB2 or GPC3) can be evaluated in human CD3 EDG-replaced mice engrafted with tumors. Our mouse model provides a novel means to evaluate the in vivo efficacy of human CD3-mediated therapy.
T cell-mediated immunotherapy is an attractive strategy for treatment in various disease areas. In this therapeutic approach, the CD3 complex is one of the key molecules to modulate T cell functions; however, in many cases, we cannot evaluate the drug candidates in animal experiments because the therapeutics, usually monoclonal antibodies specific to humanCD3, cannot react to mouse endogenous Cd3. Although immunodeficientmice transfused with human hematopoietic stem or precursor cells, known as humanized mice, are available for these studies, mice humanized in this manner are not completely immune competent. In this study we have succeeded in establishing a novel mouse strain in which all the three components of the Cd3 complex - Cd3ε, Cd3δ, and Cd3γ - are replaced by their human counterparts, CD3E, CD3D, and CD3G. Basic immunological assessments have confirmed that this strain of humanCD3EDG-replaced mice are entirely immune competent, and we have also demonstrated that a bispecific antibody that simultaneously binds to humanCD3 and a tumor-associated antigen (e.g. ERBB2 or GPC3) can be evaluated in humanCD3EDG-replaced mice engrafted with tumors. Our mouse model provides a novel means to evaluate the in vivo efficacy of humanCD3-mediated therapy.
T cells are a type of lymphocytes that play a central role in adaptive immunity along with B cells. There are various types of T cells, such as helper, cytotoxic, regulatory T cells, etc., each of which has distinct characteristics and functions in the overall immune system123. The CD3 complex, a common surface marker on T cells, has important functions not only as an essential component in forming the T cell receptor (TCR)-CD3 complex, but also as an external signal transducer; therefore, the CD3 complex is one of the target molecules to modulate T cell functions. The first antibody to humanCD3 to be approved was OKT3, which was developed to prevent rejection after organ transplantation45. Teplizumab and otelixizumab were then developed as second generation antibodies to CD3 to treat autoimmune type I diabetes567. More recently, novel therapeutic approaches have been developed for antitumor treatment using bispecific antibodies for humanCD3 and a tumor-associated antigen (TAA) to simultaneously activate effector T cells and redirect them to the tumor cells. A large number of these bispecific antibodies that target humanCD3 are already moving into the clinical phase — indeed, some are already approved — and the number is expected to increase in the near future8910.Most therapeutics that are being developed to target CD3 are molecularly targeted drugs, such as monoclonal antibodies that are highly specific to humanCD3. It is therefore difficult to evaluate such therapeutics in preclinical examinations with animal models, because interspecies sequence preservation is relatively low in the extracellular domains of CD3ε (47% homology between human and mouse at the amino acid level, CD3δ (57% homology between human and mouse), or CD3γ (60% homology between human and mouse) (Supplementary Table S1 lists accession numbers and URL addresses for each protein). Although the laboratory mouse is an excellent experimental animal, therapeutics specific to humanCD3 cannot effectively activate mouse effector T cells via their endogenous CD3 complex. Accordingly, an experimental animal model suitable for evaluating humanCD3–specific therapeutics needs to be developed. In general there are two possible approaches to humanize CD3 in mice.One approach is humanization by recapitulating the human hematopoietic system in immune-deficient mice111213. These mice have a donor-derived human immune system that includes effector T cells. However, it is well known that several types of immune cells cannot develop and maturate normally in these mice121314. Even though maturation of innate immune cells can be substantially improved by humanizing several cytokine genes, as Rongvaux et al. reported15, their adaptive immune function cannot be fully recovered, mainly because the major histocompatibility complexes (MHC) of the host cells and the humandonor T cells are mismatched, which severely hampers the educational process and the peripheral survival of human T cells16. Suzuki et al. reported that a transgenichumanMHC molecule, HLA-DR, taken from donors with compatible HLA type was effective for recapitulating the human adaptive immune system17. However, preparing a wide variety of HLA transgenic mice compatible with each donor HLA type would be a laborious challenge in large scale experiments. Another approach is to establish transgenic mice expressing the humanCD3 complex. Of the three components in the CD3 complex, CD3ε is known to play the prerequisite role in formation and function of the TCR-CD3 complex, because Cd3e-knockout mice completely lack peripheral T cells, due to the blockade in early thymocyte development181920. HumanCD3ε (CD3E) transgenicmouse strains have already been reported21, but the number of thymocytes in these humanCD3Etransgenic mice is severely reduced. The degree of thymocyte depletion correlated with transgene copy numbers, and a higher transgene copy number resulted in complete loss of T cells21. Therefore, these humanCD3Etransgenicmouse strains would not be appropriate models to evaluate CD3-mediated therapeutics. From this evidence we speculated that the expression level of transgenicCD3E in humanCD3E single transgenic mice would have to be precisely controlled and, furthermore, even if humanCD3Eexpression could be appropriately controlled, its coexistence with endogenous Cd3e could affect the normal formation of TCR-CD3 complexes, because a highly complicated combination of the CD3 components would form on the T cells (as depicted in Supplementary Fig. S1), and this unnatural combination may result in relatively fewer T cells. Moreover, we hypothesized that affinity or compatibility of CD3E with the other two components, CD3 delta (CD3D) and CD3 gamma (CD3G), would be critical to form a normal CD3 complex.In this study we have successfully established a novel mouse strain in which the entire CD3 components, i.e. CD3E, CD3D, and CD3G (referred to as CD3EDG in this paper) were genetically humanized. This mouse strain has shown normal T cell development and maturation. Several immunological assessments in vitro and in vivo have proved that their immune functions, including the T cell functions, are normal. We expect that our mouse strain will contribute to developing humanCD3–mediated therapeutics.
Results
Establishment of mice with entirely humanized CD3E, CD3D, and CD3G
The vector construction and recombination strategy used to establish entirely humanized CD3EDG–replaced mice are depicted in Fig. 1A and B. Several clones of C57BL/6N (B6) mouse embryonic stem (ES) cells (clones 1C3, 2A4, 3B1, 4HH3, and 8I12) that had been successfully recombined after two rounds of recombination were microinjected to BALB/cA mouse blastocysts to make chimeric mice. Male chimeric mice were bred with female B6 mice to obtain their offspring with a knockout allele for the entire mouseCd3edg and a humanCD3EDGtransgenic allele. After breeding the offspring from these five ES clones, five strains of endogenous Cd3edg homozygous knockout with entire humanCD3EDGtransgenic mice (referred to as humanCD3EDG–replaced mice), lines 1C3, 2A4, 3B1, 4HH3, and 8I12, were established. Representative results of genotyping PCR are shown in Fig. 1C. Neither Cre nor Dre vectors were integrated in the mouse genome. HumanCD3EDG–replaced mice were obtained in accordance with Mendelian laws. No apparent gross abnormalities were observed in any strains of humanCD3EDG–replaced mice. The Cd3edg–knockout mice (referred to as Cd3edg−/− mice) obtained in this breeding process have no apparent gross abnormalities other than in the immune system. These mouse lines were listed in Supplementary Table S2.
Figure 1
Schematic representation of the humanization strategy for CD3E, CD3D, and CD3G.
(A) A vector targeting Cd3 edg was constructed by inserting loxP and Rox with neo and hyg cassette on a BAC genomic clone. Correctly targeted ES cell clones with the Cd3 edg–targeting vector had the primary targeted allele. Next, mouse Cd3 edg genomic region flanked by two loxP sequences and the hyg cassette flanked by two Rox sequences were deleted by Cre and Dre recombinase. Arrows, PCR primers for genotyping. (B) Human CD3 EDG transgenic vector was introduced to primary targeted ES cell clones at the same time as the Cd3 edg deletion described above. Arrows, PCR primers for genotyping. (C) A representative result of genotyping to confirm deletion of endogenous Cd3 edg locus and integration of the human CD3 EDG transgene. Information of the primer set to detect each allele is listed in Supplementary Table S3. Wild allele and the disrupted allele for mouse Cd3 edg were detected as signals of 0.8 kb and 1.4 kb, respectively. The human CD3 EDG transgene was detected as a signal of 5.5 kb. Numbers above each gel denote the mouse genotypes, (1) wild-type (mCd3 edg+/+), (2) mCd3 edg+/−, hCD3 EDG Tg, (3) mCd3 edg+/+, hCD3 EDG Tg, (4) mCd3 edg+/−, hCD3 EDG Tg, (5) mCd3 edg−/−, hCD3 EDG Tg (human CD3 EDG–replaced), and (6) mCd3 edg+/−. This figure combines images cropped from the original gel electrophoresis images, which are shown in Supplementary Fig. S2A and B. (D) Representative results of RT-PCR analysis for mouse Cd3 edg or human CD3 EDG expression in the blood cells. This figure combines images cropped from the original gel electrophoresis images, which are shown in Supplementary Fig. S3A–E.
Establishment of humanized CD3E transgenic mice
As we predicted from the previous publication by Wang et al.21, it was difficult to obtain a transgenicmouse with an appropriate humanCD3Eexpression level. In total, seventeen founders were obtained by pronuclear DNA microinjection or electroporation to mouse ES cells of the humanCD3Etransgenic constructs. The humanCD3E transgene was transmitted from all founders to their offspring to establish 17 lines of transgenic mice. Of these lines, one line of the transgenic mice exhibited a desirable response in an in vitro cytotoxicity assay (data not shown), in which splenocytes from transgenic mice were incubated with a cell line expressing the TAA and a bispecific antibody to both humanCD3 and the TAA. This line of transgenic mice (referred to as hCD3ETgmice in this paper) was compared with humanCD3EDG–replaced mice for further investigation. The characteristics of the transgenicmouse lines established in this study have been listed in Supplementary Table S2.
Transgene expression of human CD3 components in the human CD3 EDG–replaced mice
Figure 1D shows representative results of the reverse transcription (RT) PCR to assess mouseCd3edg and transgenichumanCD3EDGexpression in blood cells of entirely humanized CD3EDGmice. In these results, endogenous mouseCd3edg was not detected in any of the lines tested. TransgenichumanCD3EDGexpression was detected in three lines, (1C3, 4HH3, and 8I12) and thus these three lines were used for further analysis, described below. On the contrary any of the transgenichumanCD3EDGexpression was not detected in remaining two lines of mice, 2A4 and 3B1.The results of immunohistochemical staining show that CD3-positive (CD3+) cells were located specifically in the T cell zones in the thymus and spleen of humanCD3EDG–replaced mice, just as they are in wild-type mice, whereas no staining was observed in any tissues from the Cd3edg−/− mice (Fig. 2). The CD3+ cells were morphologically normal lymphocytes. A small number of CD3+ cells sporadically distributed in all the organs of humanCD3EDG–replaced mice were morphologically normal lymphocytes, as were those of wild-type mice (Table 1 and Supplementary Fig. S4). No ectopic CD3expression was observed in any tissues of the humanCD3EDG–replaced mice, other than in lymphocytes, as far as we examined.
Figure 2
Immunohistochemical staining for CD3 in (A) the thymus and (B) the spleen. The T cell zone in each tissue was specifically stained for CD3 in human CD3 EDG–replaced mice and in wild-type mice. No staining was detected in the tissues of Cd3 edg−/− mice. wt, wild-type mice; mCd3 edg−/−, mouse Cd3 edg knockout mice; hCD3E Tg, human CD3E transgenic mice; 4HH3, 8I12 and 1C3 indicate the three different strains of human CD3 EDG–replaced mice; M, medulla; C, cortex; P, periarteriolar lymphoid sheaths (PALS); F, follicles; R, red pulps; In mCd3 edg−/−, the boundary between cortex (C) and medulla (M) was not clear in either the thymus or the spleen.
Table 1
Results of immunohistochemical staining for CD3 in mouse tissues.
1)Other tissues: liver, kidney, lung, heart, and adrenal gland.
Basic characteristics of the human CD3 EDG–replaced mice
The three lines of humanCD3EDG–replaced mice (1C3, 4HH3, and 8I12), the Cd3edg−/− mice, and the hCD3ETgmice were not significantly different in body weight (data not shown) or spleen weight (Fig. 3A) compared to wild-type mice. No anatomical abnormalities were observed in their tissues except in the thymus (data not shown). Both Cd3edg−/− mice and hCD3ETgmice have apparently atrophic thymuses. Averages of thymus weights in Cd3edg−/− mice and hCD3ETgmice were decreased by 25% and 41% that of wild-type mice, respectively. Averages of thymus weights in the three humanCD3EDG–replaced mouse lines (1C3, 4HH3, and 8I12) appeared to be, respectively, 88%, 63%, and 57% that of the wild-type mice (Fig. 3B). Of the three lines of humanCD3EDG–replaced mice, thymus weights in one line (1C3) were similar to those in wild-type mice (Fig. 3B) and thymus weights in the other two lines (8I12 and 4HH3) were significantly lower than those in wild-type mice. Although thymus sizes varied between the transgenic lines, all three lines (1C3, 4HH3, and 8I12) of humanCD3EDG–replaced mice had morphologically normal thymuses (data not shown). Total cell numbers either in the spleens or the thymuses of humanCD3EDG–replaced mouse line 1C3 were not significantly different from those in wild-type mice (Supplementary Fig. S5).
Figure 3
Weight of (A) spleens and (B) thymuses. Organ weight is shown as a ratio to body weight (n = 4, each genotype). Data are represented as mean ± s.d. In bars marked with different letters (a b, c, and d) the data sets are significantly different by Tukey-Kramer’s HSD tests, P < 0.05. Detailed data on p values between all combinations of genotypes are shown in Supplementary Tables S5A and B. wt, wild-type; mCd3 edg−/−, mouse Cd3 edg knockout mouse; 1C3, 4HH3, and 8I12 indicate the strain names of human CD3 EDG–replaced mice; hCD3E Tg, human CD3E transgenic mouse.
Splenocyte characteristics in the human CD3 EDG–replaced mice
We analyzed lineage marker expression of T and B cells in the splenocytes of humanCD3EDG–replaced mice, and compared the expression profiles with those in hCD3ETgmice and wild-type mice. Flow cytometric analysis demonstrated that humanCD3+ cells were detected in splenocytes in three lines of humanCD3EDG–replaced mice (1C3, 8I12, and 4HH3) (Fig. 4A). Certainly, mouseCd3+ cells were not detected in these mice (Fig. 4B). Of these three lines, the line 1C3 showed the highest expression of humanCD3, similar to the level of mouseCd3+ cells in wild-type mice (Fig. 4A and B). These results clearly demonstrated that mouseCd3 was successfully replaced with humanCD3 in our humanCD3EDG–replaced mice. By contrast, humanCD3+ cell populations in hCD3ETgmice were much lower than those in humanCD3EDG–replaced mice. MouseCd3+ cell populations were lower in hCD3ETgmice than those in wild-type mice, even though hCD3ETgmice have an intact endogenous Cd3edg genomic locus. These results are compatible with the description by Wang et al.21. Populations of B220+ cells, which are mainly expressed by the B lymphocytes, in all three lines of humanCD3EDG–replaced mice were similar to those in wild-type mice (Fig. 4C), whereas B220+ cells in Cd3edg−/− mice and in hCD3ETgmice were greater in number than those in wild-type mice. The cause of these increased populations of B220+ cells remains to be investigated, but we speculated that there might be a redundant mechanism that maintains the spleen tissue structure in response to T cell depletion or reduction.
Figure 4
Representative results of a flow cytometric analysis of human CD3 EDG–replaced mice, Cd3 edg−/−, and wild-type mice.
Distribution of populations of (A) human CD3, (B) mouse CD3, (C) B220, and (D) mouse CD4- or CD8-single positive cells were analyzed using splenocytes prepared from each mouse genotype. Numbers in the histogram or quadrants indicate percentage within the gated cells. wt, wild-type mice; mCd3 edg−/−, mouse Cd3 edg knockout mice; 1C3, 4HH3 and 8I12 indicate the strains of human CD3 EDG–replaced mice; hCD3E Tg, human CD3E transgenic mouse. All studies were representative of two to three experiments.
In all three lines of humanCD3EDG–replaced mice, single positive cell populations of CD4 T cells or CD8 T cells were detected (Fig. 4D). Of the three lines, the matured T cell populations in line 1C3 were most similar to those in wild-type mice. HumanCD3 derived from transgene was co-expressed with TCR beta in the 1C3 line of humanCD3EDG–replaced mice (Supplementary Fig. S6A). The percentage of matured T cell populations, i.e. CD3+CD4+ and CD3+CD8+ cells, in the 1C3 line were similar to those in wild-type mice (Supplementary Fig. S6B and C). On the other hand, neither CD4+ nor CD8+ cells were detected in Cd3edg−/− mice, and populations of CD4+ or CD8+ cells in hCD3ETgmice were decreased to about half the levels seen in wild-type mice. According to the results above, we selected the 1C3 line of humanCD3EDG–replaced mice.
Response of splenocytes to mitogenic stimulation
According to the results of flow cytometric analysis, not only T cell depletion but also abnormally increased populations of B cells were observed in the spleen of Cd3edg−/− mice (Fig. 4C). Thus, we needed to confirm that humanization of CD3EDG would not affect development and proliferation of B cells. Therefore, we examined the proliferative activity of splenocytes in response to not only T cell mitogen but also B cell mitogen using phytohaemagglutinin (PHA) as a T cell mitogen (Fig. 5A) and lipopolysaccharide (LPS) as a B cell mitogen (Fig. 5B). There was no significant difference in responses to PHA between wild-type mice and humanCD3EDG–replaced mice, whereas proliferative activity was significantly reduced in Cd3edg−/− mice. Although the response observed in Cd3edg−/− mice was higher than that in the unstimulated control, we suppose that this would be due to the response by immune cells other than mature T cells in the spleen, because PHA does not exclusively stimulate T cells, but also B cells, as previously reported22. As for LPS, substantially similar dose-dependent proliferative responses were observed in humanCD3EDG–replaced mice, Cd3edg−/− mice, and wild-type mice.
Figure 5
Proliferative response to mitogen stimulation.
Splenocytes were cultured (A) for 3 days stimulated with 1.0 μg/mL of PHA (red bar) or without stimulation (blue bar) and (B) for 2 days stimulated with 0.1 (red bar), 1.0 (green bar), or 10.0 μg/mL (purple bar) of LPS or without stimulation (blue bar). Splenocyte proliferation was analyzed by MTS assay (Promega), and the results indicated the mean absorbance at 490 nm. Data are represented as mean value ± s.e.m (n = 8). (C) Evaluation of the cytokine production with PHA stimulation. Splenocyte cells were stimulated with 1.0 μg/mL of PHA and the culture supernatants were harvested 3 days after stimulation. Cytokine levels (pg/mL) of IFN gamma and IL2 in culture medium were measured using Cytometric Bead Array (BD Biosciences). Data is significantly different compared to wild type mice. (*P < 0.05, **P < 0.0001 by Dunnett’s test for multiple comparisons.) Data are shown as dot plots (n = 8). wt, wild-type mice; mCd3 edg−/−, mouse Cd3 edg knockout mice; hCD3 EDG-replaced, human CD3 EDG–replaced mice (1C3).
To evaluate cytokine production related to T helper cells, the splenocytes were stimulated with PHA, and the cytokine concentrations in the culture supernatants were assessed (Fig. 5C). As a result, IFN gamma and IL2 in humanCD3EDG–replaced mice were detected at similar levels to those in wild-type mice. In contrast, these cytokines were produced very slightly in Cd3edg−/− mice. These results indicate that humanCD3EDG–replaced mice have immunological competency in mitogenic stimulations.Next, we examined whether T cells in humanCD3EDG–replaced mice would respond to stimulation with agonistic antibodies specific to humanCD3 and mouseCd3, and compared the results with the responses to agonistic antibodies specific to mouseCd3 and humanCD3 in wild-type mice. As a result, splenocytes from humanCD3EDG–replaced mice could proliferate (Fig. 6A) and produce cytokines in response to the humanCD3 antibody (Fig. 6C), but did not respond to the mouseCd3 antibody. Meanwhile, splenocytes from wild-type mice could respond to the mouseCd3 antibody (Fig. 6B and D), but could not respond to the humanCD3 antibody.
Figure 6
Representative results of an MTS assay to evaluate cell proliferation after stimulation with an antibody specific to mouse or human CD3.
Splenocytes were stimulated with anti-human CD3 antibody (A,C) and anti-mouse CD3 antibody (B,D). After 3 days stimulation, splenocyte proliferation was analyzed by MTS assay (Promega) (A,B). Cytokine productions were determined in human CD3 EDG–replaced mice, Cd3 edg−/− mice, and wild-type mice (C,D). The culture supernatants were harvested 3 days after stimulation and cytokine levels (pg/mL) of IFN gamma, TNF alpha, IL6, IL10, IL4, and IL2 in culture medium were measured using Cytometric Bead Array (BD Bioscience). Data are represented as mean value ± SEM (n = 8). wt, wild-type mice; mCd3 edg−/−, mouse Cd3 edg knockout mice; hCD3 EDG-replaced, human CD3 EDG–replaced mouse line 1C3.
Specific antibody production in response to immunization with an external antigen, ovalbumin (OVA)
After the second immunization of OVA with Freund adjuvant, both the OVA-specific immunoglobulin (Ig) E- and Ig G1-class antibodies were detected in the serum of humanCD3EDG–replaced mice (Fig. 7). The levels of OVA-specific IgE and IgG1 titers were similar to those in wild-type mice. In contrast, neither OVA-specific IgE nor IgG1 titers were detected in the serum of Cd3edg−/− mice. These results indicate that humanCD3EDG–replaced mice respond to immunization with external antigens by producing normal levels of antibody.
Figure 7
Serum titers of OVA-specific IgE- and IgG1-class antibodies.
Mice were immunized with OVA twice, 4 weeks apart. Blood samples were collected a week after the second immunization. Each bar represents serum concentration of OVA specific-IgG1 or IgE of individual mice. wt, wild-type mice; mCd3 edg−/−, mouse Cd3 edg knockout mice; hCD3 EDG, human CD3 EDG–replaced mice; #1C3 and #8I12 indicate strains of human CD3 EDG–replaced mice; hCD3E Tg, human CD3E transgenic mouse.
T cell activation with hCD3-TAA bispecific antibodies in human CD3 EDG–replaced mice
We tested T cell–dependent cellular cytotoxicity (TDCC) using a T cell–redirecting antibody (TRAB). In this TDCC assay, the effector cells were spleen cells of humanCD3EDG–replaced mice and the target cells were Hepa1-6/hGPC3/HER2 cells, in which humanglypican-3 (GPC3) and erb-b2 receptor tyrosine kinase 2 (HER2) are significantly expressed in Hepa1-6mousehepatocellular carcinoma (Fig. 8A and B). TRABs bispecific to hCD3 and either HER2 or hGPC3 showed TDCC (described as cytotoxicity (%) calculated by equation (1) in the Methods section) with effector cells from humanCD3EDG–replaced mice (Fig. 8C), but did not show TDCC with effector cells from wild-type mice (Fig. 8D). On the other hand, a TRAB bispecific to mCD3 and hGPC3 showed TDCC with effector cells from wild-type mice, but did not show TDCC with effector cells from humanCD3EDG–replaced mice. These results demonstrated that TDCC induced by TRABs is dependent on the combinations of antibody with target CD3 and on the genotype of effector cells. To confirm the activation of T cells, we then examined the expression levels of CD69 (an early marker of T cell activation), CD25 (a late marker of T cell activation), CTLA-4 (CD152), and ICOS (CD278). As shown in Fig. 9A–D, CD25 and CD69expression increased on T cells derived from humanCD3EDG–replaced mice treated with TRABs bispecific to hCD3 and either HER2 or hGPC3, whereas when a TRAB bispecific to mCD3 and hGPC3 was used, CD25 and CD69expression was increased on T cells derived from wild type mice, but not on T cells derived from humanCD3EDG–replaced mice. Changes in CTLA-4 and ICOS expression were not observed clearly in these samples (data not shown).
Figure 8
TRAB-mediated killing by splenic T cells of human CD3 EDG–replaced mice.
Surface expression of (A) GPC3 and (B) HER2 was determined on Hepa1-6/hGPC3/HER2 cells by FACS. T cells were extracted from the spleens of (C) human CD3 EDG–replaced mice or (D) C57BL/6 mice. In vitro killing activity of Hepa1-6/GPC3/HER2 cells was tested using human CD3 TRABs specific to hGPC3 or HER2, and a mouse CD3 TRAB specific to hGPC3. E:T = 40:1 Assay time: 72 hours. In vitro cytotoxicity was monitored by xCELLigence.
Figure 9
Target-dependent T cell–activation.
The expression levels of activation markers CD25, CD69, on (A,C) CD4+ or (B,D) CD8+ T cells were determined by flow cytometry. T cells were prepared from the in vitro tumor cell killing assay in Fig. 8, at the 72 hours timepoint. WT, wild type mouse; TG, human CD3 EDG–replaced mouse; no ab, without antibody administration.
When the antitumor effect of the TRAB to HER2 was examined in a humanCD3EDG–replaced mouse model engrafted with Hepa1-6/hGPC3/HER2 cells, the antitumor effect was significant, with 149% tumor growth inhibition (TGI, calculated by equation (2) in the Methods section) at 28 days after tumor implantation (Fig. 10A). The antitumor effect of the PD-L1 antibody was also observed in a humanCD3EDG–replaced mouse model engrafted with Hepa1-6/hGPC3 cells. The antitumor effect was significant, with 75% TGI at 37 days after tumor implantation (Fig. 10B).
Figure 10
A TRAB bispecifically targeting hCD3 and HER2 or anti-PD-L1 antibody inhibits in vivo growth of tumor in the human CD3 EDG–replaced mouse model.
A total of 1 × 107 Hepa1-6/hGPC3/HER2 cells or Hepa1-6/hGPC3 were inoculated together with 50% matrigel-matrix (BD Bioscience). (A) Mice were treated with 5 mg/kg i.v. doses of the TRAB (n = 4) or the vehicle (n = 5) on Day 11 after tumor inoculation. (B) Mice (n = 5) were injected with a 10-mg/kg i.v. dose of anti-PD-L1 antibody on Days 21 and 24. Arrows show the time of antibody injection. HER2/hCD3-TRAB: bispecific antibody to hCD3 and HER2 (*P < 0.05 by Wilcoxon test).
Discussion
This report explains how we successfully established a novel mouse strain that has an entirely humanized CD3 complex by disrupting the endogenous genome covering Cd3e, Cd3d, and Cd3g and simultaneously introducing a complete genomic region of humanCD3E, CD3D, and CD3G. The most important advantage of our humanCD3EDG–replaced mouse strain is in immune competence. Our mouse strain is immunologically normal in tests so far. First, neither T cell reduction nor thymus hypoplasia were observed in the humanCD3EDG–replaced mouse line 1C3 (Fig. 3B and Supplementary Fig. S5), whereas both abnormalities were previously reported in hCD3ETgmice and also reconfirmed in this study (Fig. 3B). The thymus weights observed in the humanCD3EDG–replaced mice varied between the transgenic lines. We speculate that there may be some subtle differences in transgene expression levels between the three lines, possibly due to the effect of some neighboring genomic elements, e.g. enhancers, suppressors, genomic structure, etc., that surround the transgene integration site of each line. Secondly, T cell differentiation into mature CD4 or CD8 single positive T cells is normal in the humanCD3EDG–replaced mice (Fig. 4D and Supplementary Fig. S6B and C). It is well known that appropriate signals from TCRs at an appropriate time are essential for normal T cell development and differentiation in the thymus23. According to an MTS assay, the T cell proliferative response is normal after several mitogen stimulations on the spleen cells (Fig. 5A and C). A species-specific agonistic antibody to CD3 can differentially stimulate splenocytes according to their genotypes (Fig. 6A–D), which demonstrates that not only has endogenous mouseCd3edg been replaced with humanCD3EDG but also humanCD3EDG functions normally on T cells in mice. Thirdly, helper T cells in our mice stimulate B cells normally to produce Ig E and Ig G1 antibodies specific to a foreign antigen, OVA (Fig. 7), indicating that Ig isotype switching is also taking place normally. It is well known that CD4+ helper T cell functions are essential, not only to produce specific antibodies but also for antibody isotype switching and affinity maturation2425. These results demonstrated that CD4+ helper T cells function normally in our humanCD3EDG–replaced mice. Although the function of regulatory T cells remains to be investigated, it is expected that they would develop and function normally because humanCD3EDG–replaced mice do not show signs of autoimmunity3. The results above clearly show that our humanCD3EDG–replaced mice are immunologically competent. We expect that our humanCD3EDG–replaced mice will contribute especially to the development of therapeutics, either antibodies for use in the extracellular domain or small molecule drugs etc. for use in the cytoplasmic domain, to treat cancer or the autoimmune diseases.Recent advances in antibody-engineering technology make it possible to develop not only target-specific therapeutics but also antibodies with various functions, such as bispecific target-binding, agonistic activity, conditional target-binding properties, and effector cell redirection826272829. Of these antibody-based therapeutics, TRABs are attracting attention in the field of cancer immunotherapy8. A TRAB is a type of bispecific antibody that can simultaneously bind to a target antigen on the tumor cell and to CD3 to activate T cells residing in the tumor through the CD3 complex, without interacting with antigen-presenting cells and thus independent of their TCR-binding specificity. Antibody engineering has been used to develop numerous biologics of this type, including the bispecific T Cell Engager (BiTE) antibodies9. For clinical trials of these therapeutic antibodies to be successful, their efficacy needs to be adequately evaluated in preclinical experiments; however, as noted earlier, interspecies sequence preservation is relatively low in the extracellular domains of either CD3ε, CD3δ, or CD3γ. In many cases, humanized mouse models, which are immune-deficient mice transfused with human hematopoietic stem or precursor cells, have been widely used for preclinical evaluation of therapeutics that specifically target human molecule(s) on blood cells, such as immune cells11121314, but these humanized mouse models are not completely immune-competent either in terms of innate immunity or adaptive immunity. To resolve the lack of immune-competent animal models for evaluating antibody-based therapeutics that target humanCD3, we examined whether our novel humanCD3EDG–replaced mouse model can be used to evaluate the in vivo efficacy of TRABs. As a result, complete growth inhibition was observed after administering a TRAB against HER2 and humanCD3 in a model engrafted with syngeneic tumor cells that express both humanHER2 and humanGPC3 (Fig. 10A), and several in vitro experiments demonstrated that the growth inhibition effect was via TDCC activity (Figs 8 and 9). Moreover, the study showed that inhibiting the immune checkpoint pathway through PD1 and PDL1 can result in growth inhibition of grafted tumor cells (Fig. 10B), which indicates that effector T cells in humanCD3EDG–replaced mice can be normally activated by immune checkpoint inhibitors.In any case, only using conventional immunodeficientmouse models would not be sufficient to precisely evaluate drug candidates. We would like to propose the importance of evaluating drug candidates in multiple humanized animal models: one is the conventional model that recapitulates the human immune system in immunodeficientmice, and another is an immune-competent mouse model like our humanCD3EDG–replaced mouse. Nowadays, numerous novel therapeutics are being developed for cancer immunotherapy and autoimmune diseases using the latest advances in drug-engineering technologies. We hope that our humanCD3EDG–replaced mice can contribute to the development of these innovative drugs in the near future.
Methods
Generation of entire human CD3E, CD3D, and CD3G–replaced mice
Bacterial artificial chromosome (BAC) genomic DNA clones that cover the entire mouseCd3 gene region (Invitrogen Clones, RPCI23.C., Clone#410N16)30 or the humanCD3 gene region were purchased from Life Technologies (Invitrogen Clones, RPCI11.C., Clone#30E1)31.A targeting vector was constructed to disrupt the entire genomic region covering mouseCd3 (Cd3e, Cd3d, and Cd3g). A BAC genomic DNA clone that covers the entire mouseCd3 gene region was used to construct the targeting vector by using Red/ET system (Gene Bridges, GmbH)3233. At first, a loxP site with neo (loxP-neo) cassette was inserted at 5′ upstream of Cd3e on the genome in the BAC clone, and simultaneously 5′ upstream region was shaved to approximately 3.5 kb as a 5′ homology arm. Next, another loxP site and a hygromycin resistance gene (hygR) cassette flanked by two Rox sites (loxP-Rox-hygR-Rox cassette) were inserted at 3′ downstream of Cd3g. Finally 3′ downstream region of Cd3g was shaved to approximately 3.4 kb as a 3′ homology arm.The vector introducing the entire humanCD3 gene (CD3E, CD3D, and CD3G) was constructed by recombination of the genomic region cloned in the BAC vector with Red/ET system. The 5′ upstream genomic region of CD3E was shaved to 6.5 kb by simultaneous insertion of a hygromycin resistance cassette. Next, 3′ downstream region of CD3G was shaved to approximately 4.2 kb by simultaneous insertion of a dual drug selection marker, which consists of a puromycin resistance gene cassette flanked with Frt and a neo cassette with a Rox site (Fig. 1B).HumanCD3EDG–replaced mouse ES cell lines were established by two rounds of recombination protocol as described below. At the first recombination, mouseCd3 targeting vector was electroporated to C57BL/6N (B6) mouse ES cells. The ES cells were selected in a culture medium containing G418. G418-resistant ES cell clones were screened by PCR protocol to confirm that both loxP-neo cassette and loxP-Rox-hygR-Rox cassette were correctly inserted in the target genomic sites. Correctly mutated ES cell clones (referred to as primary mutant ES cell clones) were expanded for the second recombination. The vector introducing the entire humanCD3EDG gene was electroporated to the primary mutant ES cell clones with Cre and Dre expression vectors. The ES cells were selected in a medium containing puromycin. Puromycin-resistant ES cell clones were screened by PCR protocol to confirm integration of the humanCD3 genomic DNA and complete the deletion of mouse endogenous Cd3 genomic region. Correctly mutated ES cell clones were injected into BALB/cA mouse (CLEA Japan, Tokyo) blastocysts to produce chimeric mice. Chimeric mice were bred with B6 females to establish humanCD3EDG–replaced mouse lines. Genotyping was performed by genomic PCR in this breeding process. Primer sets, used for endogenous mouseCd3 locus, mouseCd3edg−/− locus and transgenichumanCD3EDG, are listed in Supplementary Table S3. After several assessments for transgene expression and basic immunological tests, we selected the 1C3 line of hCD3 EDG–replaced mice (officially named C57BL/6N-Del(9Cd3e-Cd3g)1Csk-Tg(CD3E, CD3D, CD3G)1Csk).
Generation of human CD3E transgenic mice
HumanCD3Etransgenic mice (official strain name: C57BL/6N-Tg(hCD3E)301Csk) were established by basically the same protocol as that described previously by Wang21, except that the vector was constructed with the Red/ET system. The genomic region, containing all the exons and introns of CD3E with 6.5 kb of 5′ upstream region and 8 kb downstream region, was separated by pulsed-field gel electrophoresis and microinjected into the pronucleus of B6 mouse–fertilized eggs.
RT-PCR for evaluation of transgenic human CD3 EDG and mouse endogenous Cd3 edg gene expression
RT-PCR analysis was performed to determine humanCD3EDG and mouseCd3edg gene expression. Total RNA samples, which were purified from mouse blood with Catrimox-14 RNA Isolation Kit (TaKaRa Bio, WA005, Japan) or NucleoSpin RNA Blood Kit (TaKaRa Bio, U0200B, Japan), were reverse-transcribed with SuperScript III reverse-transcriptase (Invitrogen) to synthesize cDNA. PCRs were performed with the gene-specific primers listed in Supplementary Table S4.
Immunohistochemical staining of CD3
Tissue samples were fixed in 10% neutralized formalin and were embedded in paraffin blocks. Antigen retrieval was performed for the tissue sections from these paraffin blocks by microwave oven for 10 min in Target Retrieval Solution (DAKO, S1699). After incubation in 30% hydrogen peroxide in methanol for 30 min to block endogenous enzyme activity, tissue sections were incubated in working solution of M.O.M.™ Mouse IgG Blocking Reagent (Vector® M.O.M.™ Immunodetection Kit) for 1 hour and then in 5%BSA/TBS buffer for 30 min. Monoclonal anti-humanCD3 (2.5 μg/mL, DAKO F7.2.38) was used as a primary antibody for incubation overnight at 4 °C. After incubation with secondary antibody, rat anti-mouse IgG heavy chain (LO-MG1-13: Abcam ab11585), biotin-labelled rabbit anti-rat IgG (5.0 μg/mL #A110-322, Bethyl), and HRP-labeled streptavidin (5.0 μg/mL, Vector SA-5740) were applied according to the standard ABC method. Tris-HCl buffer with 0.05% 3.3′-diaminobenzidine (DAB) in 0.03% hydrogen peroxide was used for staining.
Flow cytometry analysis
Primary splenocytes were isolated from each mouse by mechanical dissociation followed by red blood–cell lysis. These splenocytes were stained with the following monoclonal antibodies: FITC labeled anti-humanCD3 (clone; UCHT1), FITC labeled anti-mouseCD3 (clone; 17A2), APC labeled CD4 (clone; RM4-5), PE labeled CD8 (clone; 53-6.7), APC-Cy7 labeled CD45R/B220 (clone; RA3-6B2). All antibodies were purchased from BD Biosciences. The expression of cell surface antigens was analyzed by flow cytometry (CyAn ADP, Beckman Colter Inc. or FACSVerse, BD Biosciences).In order to check target-dependent T cell–activation, the expression levels of activation markers were analyzed by flow cytometry (BD FACSVerse) after in vitro tumor cell killing assay. These T-cells were stained with the following monoclonal antibodies: BUV395 labeled anti-mouseCD45 (BD Horizon, Clone; 30-F11), PE-CF594 labeled CD4 (BD Horizon, clone; RM4-5), perCP-Cy5.5 labeled CD8 (BD Horizon, clone; 53-6.7), FITC labeled CD25 (BD Pharmingen, clone; 7D4), APC/Cy7 labeled CD69 (BD Pharmingen, clone; H1.2F3).
Splenocyte proliferation and cytokine production
Splenocytes were cultured in complete RPMI1640 medium (Thermo Fisher) containing 10% fetal bovine serum and supplemented with PHA or LPS. These mitogens were purchased from SIGMA. For splenic T cell–stimulation via CD3, splenocyte cells were cultured on a plate coated with antibody to mouseCd3 (145-2C11) or antibody to humanCD3 (HIT3a). These antibodies were purchased from BD Biosciences. Two or 3 days after stimulation, splenocyte proliferation was analyzed by MTS assay (Promega) and culture supernatants were analyzed for cytokine concentrations using Cytometric Bead Array (BD Biosciences).
Immunization with an external antigen, OVA
An emulsion prepared by mixing chickenOVA and Freund’s complete adjuvant (OVA/FCA emulsion) was used for first immunization. Each mouse was subcutaneously injected with the OVA/FCA emulsion. Four weeks later, each mouse was immunized with OVA again, similarly to the first immunization except for using Freund’s incomplete adjuvant. One week after the second immunization, whole blood samples were collected from the inferior vena cava of the mice under isoflurane anesthesia. Serum levels of the OVA-specific immunoglobulin (Ig) E and Ig G1 were determined using the DS Mouse IgE ELISA (OVA) kit (DS Pharma, Japan) and MouseOVA-IgG1 ELISA kit (Shibayagi, AKRIE-040, Japan), respectively, according to the manufacturer’s protocols.
Antibodies
A bispecific antibody to HER2 and hCD3 was generated by Fab arm exchange using anti-HER2 antibody (trastuzumab) and anti-humanCD3 antibody (UCHT1). Bispecific antibody against hGPC3 and hCD3 was manufactured as full length human IgG4 by applying technologies for light chain commonization, heavy chain heterodimerization, and isoelectric point modification [Ishiguro, T. et al. Manuscript submitted]. Bispecific antibody against hGPC3 and mCD3 was generated by Fab arm exchange using anti-GPC3 antibody (GC33) and anti-mouseCD3 antibody (2C11). Anti-mousePD-L1 antibody was purchased from BioXcell (clone: 10F.9G2).
Cells and culture conditions
Hepa1-6/hGPC3/HER2 cells (ATCC), which overexpressed hGPC3 and HER2 in Hepa1-6, were cultured in RPMI1640 (SIGMA) supplemented with 10% FBS (SIGMA), 0.6 mg/mL G418 (Nacalai Tesque), and 0.5 mg/mL Zeocin (Nacalai Tesque).
In vitro cytotoxicity and analysis of T-cell activation
In vitro cytotoxicity assays (TDCC) were monitored by xCELLigence Real-Time Cell Analysis (RTCA) system (ACEA Biosciences). The target cells (2.5 × 103 cells) and spleen cells (1 × 105 cells) from humanCD3EDG–replaced mice and wild-type (C57BL/6) mice were mixed with or without TRAB for 72 hours. The percentage of cytotoxicity was calculated as follows:where A was the mean cell index of wells without TRAB; B was the mean cell index of wells with TRAB. Baseline was normalized as 1.At the end of incubation, the cells were collected from the plate. Cells were stained with mouseCD4 (BD Horizon), CD8, CD25, CD69, CD152 (BD Pharmingen), and CD278 (eBioscience) and analyzed by flow cytometer.
In vivo models
The effects of TRABs or anti-PD-L1 antibody34 were tested in humanCD3EDG–replaced mice. Dosing and monitoring were performed in accordance with guidelines from the Institutional Animal Care and Use Committee at Chugai Pharmaceutical, Co., Ltd. HumanCD3EDG–replaced mice were subcutaneously inoculated with 10 million cells. Five mg/kg TRABs or 10 mg/kg anti-PD-L1 antibody were administered by i.v. injection in the tail vein. TGI was calculated as follows:where T is tumor volume in the treated group at measurement, T0 is tumor volume in the treated group at baseline, C is tumor volume in the control group at measurement, and C0 is tumor volume in the control group at baseline.
Guidelines
Entire humanCD3EDG–replaced mice and humanCD3Etransgenic mice were generated in accordance with the Guidelines for the Care and Use of Laboratory Animals and the Ethical Guidelines for Research Using Human Specimens at Chugai Pharmaceutical Co. Ltd.Protocols for the animal experiments, including generation of humanCD3EDG–replaced mice and humanCD3Etransgenic mice, RT-PCR for evaluation of transgenichumanCD3EDG and mouse endogenous Cd3edg gene expression, immunohistochemical staining of CD3, flow cytometry analysis, splenocyte proliferation and cytokine production, immunization with an external antigen, OVA, in vitro cytotoxicity and analysis of T-cell activation, and in vivo models, were approved by the Care and Use of Laboratory Animals at Chugai Pharmaceutical Co. Ltd.
Statistical analysis
Statistical analysis was performed using JMP 9.02 (SAS Institute Japan, Tokyo, Japan). Statistical significance in thymus and spleen weights were determined by Tukey-Kramer’s HSD test and MTS values were determined by nonparametric comparisons with control using the Dunn method for joint ranking. Tumor growth inhibition data was determined by Wilcoxon test. P < 0.05 was regarded as statistically significant.
Additional Information
How to cite this article: Ueda, O. et al. Entire CD3ε, δ, and γ humanized mouse to evaluate humanCD3–mediated therapeutics. Sci. Rep.
7, 45839; doi: 10.1038/srep45839 (2017).Publisher's note: Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
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