Layered immune system development in mice and humans

IF 7.5 2区医学 Q1 IMMUNOLOGY

Immunological Reviews Pub Date : 2023-03-24 DOI:10.1111/imr.13198

Kenneth Dorshkind, Gay Crooks

{"title":"Layered immune system development in mice and humans","authors":"Kenneth Dorshkind, Gay Crooks","doi":"10.1111/imr.13198","DOIUrl":null,"url":null,"abstract":"It is fitting to begin the introduction to this volume of Immunological Reviews by discussing a 1986 review in this journal from Herzenberg and colleagues which introduced the concept of layered immune system development.1 That contribution summarized functional differences between conventional B cells, which participate in adaptive immune responses and constitute the majority of B lymphocytes in mouse tissues, and a minor population of Ly-1 B cells that are innate-like effectors. Ly-1 B cells are now referred to as B-1 B cells while conventional B cells are designated as B-2 B cells. Based on data showing that neonatal bone marrow cells reconstituted B-1 B cells in irradiated recipients but adult bone marrow could not do so, B-1 and B-2 B cells were proposed to be distinct developmental lineages. This view was later reinforced by data from Hardy and Hayakawa, who discovered B-1 B cells in Leonore Herzenberg's laboratory,2 showing that fetal liver pro-B cells could reconstitute cells with a B-1 B cell phenotype in immunodeficient mice while adult bone marrow cells failed to do so.3The developmental distinctions between B-1 and B-2 B cells were the basis for a now widely cited 1989 commentary in Cell by Leonore and Leonard Herzenberg in which they presented the basic tenets of layered immune system development.4 Their layered immune system hypothesis proposed that the various types of lymphocytes that constitute the adult immune system developed in waves from distinct progenitors that emerged at different times during development. B-1 B cells emerged in the first, most primitive wave of development along with fetal erythrocytes and selected γδ T cells. A subsequent wave produced the so-called Ly-1 B sister population. The B-1 B cells in these two waves would now be referred to as B-1a and B-1b B cells which are known to function differently.5-7 A third wave generated conventional B and T cells from self-replenishing progenitors in postnatal bone marrow throughout life. Studies conducted over the past 30 years have validated many aspects of the layered immune system hypothesis and suggested that the layering of immune system development is more extensive than initially envisioned by the Herzenbergs. The contributions that form this edition of Immunological Reviews provide a comprehensive summary of the evidence for developmental layering of many if not all lineages of the innate and adaptive immune system.There is no general consensus regarding the number of waves of immune and hematopoietic system development that occur in the fetus and adult. However, the emergence of hematopoietic stem cells (HSCs) and lymphoid and myeloid progenitors in mice can be considered in the context of three broad developmental windows.1. Pre HSC hematopoiesis: It has been recognized for decades that the extra-embryonic yolk sac is a site of early hematopoiesis and that red blood cells develop in that tissue prior to the emergence of HSCs,8, 9 which in the mouse occurs at embryonic day (E) 10.5. However, progenitors with myeloid potential also arise in the early yolk sac, and it is now established that their macrophage progeny are retained long-term in the adult as brain microglia, liver Kupffer cells, skin Langerhans cells, and alveolar macrophages.10, 11 The erythro-myeloid progenitors (EMPs) that arise as early as E8.25 in the yolk sac also generate mast cells, some of which are maintained in the adult. The contributions from Kobayashi and Yoshimoto12 and from Chia et al.13 address the origin of mast cell progenitors during this early wave of yolk sac hematopoiesis as well as at later stages of development. In addition to discussing the origins of mast cells in different waves of hematopoiesis, the comprehensive chapter from Chia et al. reviews the impact of mast cells on various developmental and pathologic processes. Their review is a must read for those interested in mast cell biology. The Herzenberg's 1989 perspective4 proposed that many perplexing aspects of myeloid development can be clarified when viewed from the perspective of layered hematopoietic development, and the information contained in these reviews indicates they were correct.Additional studies in mice surprisingly revealed that in addition to erythroid and myeloid cells, progenitors in the pre-HSC yolk sac can generate αβ and γδ T cells and B-1, but not B-2, B cells. Many of these revelations were initially made by Momoko Yoshimoto in collaboration with Mervyn Yoder and subsequently in her own independent laboratory and are summarized in the review by Kobayashi and Yoshimoto.12 The degree to which B and T cells derived from this initial wave of lymphopoiesis contribute to fetal and/or adult immunity remain to be determined.2. Mid-gestation hematopoiesis: Multiple hematopoietic populations are present in the mid-gestation fetus as discussed by Soares-da-Silva et al.14 and other reviews herein. These include HSCs, thymus seeding progenitors, B-1 and B-2 progenitors, and innate lymphoid progenitors (ILCs). The possibility that ILCs, and those in the ILC3 family in particular, emerge in separable waves of development are discussed in detail in the chapter from Van de Pavert15It is not always easy to define the origin of the various progenitors present in the mid-gestation fetus, as some may have been generated in the pre-HSC period described above while others are likely the progeny of HSCs that emerge from hemogenic endothelium during this mid-gestation period. Further complicating the picture are recent studies concluding multi-potential progenitors (MPPs) arise from hemogenic endothelium in a wave(s) of development distinct from that of HSCs.16, 17 A major challenge will be to resolve the number of waves of lymphoid and myeloid development that arise within narrow time frames during mid-gestation and catalog the various stem and progenitor populations that are produced. The reviews from Montecino-Rodriguez and Dorshkind18 and Soares-da-Silva et al.14 which define several distinct waves of B and T cell development are relevant in this regard.3. Adult hematopoiesis: A distinguishing characteristic of this period is the production of conventional B and T cells, while the generation of various innate-like lymphocytes either does not occur or is highly attenuated. For example, although γδ T cells can be generated in the adult thymus, the production of those that utilize the Vγ3 family is restricted to fetal hematopoiesis. Furthermore, the potential of adult marrow stem and progenitor cells to produce B-1a B cells is limited as discussed in reviews from Montecino-Rodriquez and Dorshkind18 and Koybayashi and Yoshimoto.12 The latter reviews discuss the controversy regarding postnatal B-1 B cell development in light of studies showing the potential of adult marrow to generate those cells. The issue is not whether B-1 B cells, and B-1a B cells in particular, can develop from precursors in adult marrow but the efficiency with which they do so, and those reviews make the point that B-1 output from adult precursors is significantly attenuated compared to fetal progenitors. It is tempting to speculate that the few B-1 B cells generated in adult marrow are the progeny of a few fetal stem and progenitor cells that survive long-term after birth.It has been suggested that adult bone marrow hematopoiesis does not adhere to the canonical model of hematopoiesis, which proposes that HSCs at the head of the hematopoietic hierarchy are responsible for all adult blood cell production. Kobayashi and Yoshimoto12 review recent results from their group and the Carmago laboratory16 indicating that the fetal derived MPPs that arise distinct from HSCs as discussed above are retained in adult bone marrow long-term and make a significant contribution to adult lymphopoiesis for up to 2 years after birth. These recent findings are interesting in view of earlier barcoding studies indicating that progenitors, and not HSCs, are responsible for most day to day blood cell production.19, 20 However, this model has been challenged.21 These observations indicate that additional studies are needed to clarify how steady state blood cell production in the adult is sustained.The results discussed above were obtained from analysis of mice, but there is evidence that layering of immune system development also occurs in humans as presented in three reviews in this issue of Immunological Reviews. Sanchez et al.22 discuss single cell sequencing results that support the existence of several distinct functional waves of γδ T cell development in the human fetal thymus. They also review the role of Lin28b and additional intrinsic and extrinsic factors in driving the fetal γδ T cell receptor repertoire in human γδ thymocytes. The contribution from Tabilas et al.23 reviews evidence that the functions of CD8 T cells in adults is linked to when they were produced. For example, CD8 T cells in neonatal mice have rapid innate-like functions and those in adult animals have slower adaptive characteristics. Their chapter provides an overview of single cell sequencing results which support the existence of distinct ontogenic populations of CD8 T cells in humans. Burt and McCune24 present a detailed review that also supports the layered development of human CD8 as well as CD4 T cells.However, whether the layering of immune system development in humans is as extensive as in mice is unclear. For example, it has been challenging to identify human B-1 B cell progenitors. Until it is possible to do so, whether these cells emerge in distinct waves, if at all, in humans remains to be determined. Sun et al.25 discuss the difficulty in definitively fate-mapping lymphoid cells in humans back to their developmental origin. As a result, they point out that, despite suggestive literature, it is difficult to conclude that human yolk sac progenitors give rise to lymphocytes in an HSC independent manner as has been shown in mice.In fact, studies of early human lympho-hematopoiesis are challenging, because it is not easy to obtain human fetal tissues, particularly at precisely timed stages of development as discussed by Burt and McCune.24 In addition, they point out that the sophisticated lineage tracing models that have been used in mice, discussed in the various chapters herein and the review from Van de Parvet15 in particular, are not available. That is why various in vitro models, including the generation of HSCs and progenitors from embryonic or induced pluripotent stem cells and systems such as the artificial thymus organ (ATO) cultures26, 27 will be important for defining the developmental potential of fetal and adult derived stem and progenitor cells as further discussed by Sun et al..25 The ATO model is a particularly powerful system as it generates the full range of human T differentiation, including production of mature CD4+ and CD8+ T cells, and allows comparisons of development from fetal and adult hematopoietic stem and progenitor cells (HSPCs). For example, in contrast to postnatal thymopoiesis, terminal deoxynucleotidyl transferase (TdT) expression is absent during T cell differentiation from pluripotent stem cells in ATOs, reflecting a previously reported property of fetal lymphopoiesis.28If multiple populations of stem and progenitor cells with distinct developmental potential arise in different waves of fetal and adult hematopoiesis, it is reasonable to assume that they will exhibit differences in gene expression. The review from Montecino-Rodriguez and Dorshkind18 discusses how the genetic regulation of mouse B and T cell development within and between waves of fetal and adult lymphopoiesis differs. There are multiple waves of murine thymopoiesis as discussed in detail by Soares-da-Silva et al.14, and MacNabb and Rothenberg29 present a masterful review that compares the transcription factor networks involved in T cell differentiation in the fetal and adult mouse thymus. Their review is distinguished by an elegant genetic analysis of genome-wide transcription data that has become available in recent years. As noted above, the single cell human sequencing studies have also revealed differences in gene expression in waves of human γδ T cell development as discussed by Sanchez et al.22At least two models can be formulated to explain the layering of immune and hematopoietic system development (Figure 1). The “Multiple Stem/Progenitor Cell model” proposes that multiple types of stem and progenitor cells with distinct developmental potential arise in overlapping waves of development. For example, Beaudin et al. identified a transient fetal HSC with the potential to produce innate-like lymphocytes (eg B-1 B cells, Vγ3+ γδ T cells) distinct from adult HSCs which primarily produced conventional B and T cells.30 Their data provide support for the Herzenberg's prediction that “several types of hematopoietic stem cells that have evolved sequentially and function at specified times during development” exist. It is interesting, particularly in view of the detailed discussion by Soares-da-Silva et al.14 about when stem cell expansion in the fetus occurs, that the fetal HSCs described by Beaudin et al. were more proliferative than adult stem cells.An alternative “Molecular Layering model” is presented in the review from Burt and McCune.24 Based on single cell sequencing of human cord blood HSPCs and T cells, those investigators concluded that the stem and progenitor cell pool in the fetus is relatively homogeneous and that, at least from the perspective of T cell development, “the transition from human fetal to adult T cell identity and function does not occur due to a switch between distinct fetal and adult lineages. Rather, recent evidence from single cell analysis suggests that during the latter half of fetal development a gradual, en masse progressive transition occurs at the level of hematopoietic stem-progenitor cells (HSPCs) which is reflected in their T cell progeny”. This model is consistent with results from a mouse study by Kristiansen et al.31 who used a cellular barcoding approach to track individual HSPCs in the fetus and adult and showed that stem cells in the fetus could generate innate-like B-1 and selected γδ T cells and this potential was lost in the adult. These differences were linked to the expression of the Lin28b RNA binding protein, which is expressed in fetal and downregulated in adult HSCs. Interestingly, re-expression of Lin28b in adult HSCs allowed them to now produce innate like B and T cells. These observations raise the question of what regulates changes in gene expression in a fetal HSPC as it takes up residence in the adult? One possibility, as discussed by Burt and McCune,24 is that HSPCs possesses an internal clock that coordinates changes in gene expression over time. Alternatively, changes in the environments stem cells occupy may trigger changes in gene expression.In some cases, it is possible to explain the existence of particular fetal progenitors with either model. For example, our group defined a murine B-1 B cell restricted progenitor which we discuss in detail in our review in this volume.32 These progenitors are primarily present in fetal tissues and only at very low levels in adult bone marrow.32 If the multiple stem/progenitor cell model is considered, B-1 progenitors could arise directly, such as in the early yolk sac or in the mid-gestation embryo, in a stem cell independent manner. They, along with B-2 B cells and various myeloid progenitors could also be the progeny of fetal MPPs or HSCs. From the perspective of the molecular layering model, B-1 progenitors could be the progeny of a homogenous population of fetal HSCs that express Lin28b. However, as the expression of Lin28b and other fetal lineage specifying genes is downregulated, stem cells no longer generate B-1 and other innate-like progenitors or do so with significantly reduced efficiency. However, in other cases only the multiple stem/progenitor model can explain experimental results. For example, if distinct populations of HSCs and MPPs that arise independent from one another exist, their origin is difficult to explain based on the molecular layering model.When attempting to reconcile data, it is important to consider that the two models are not mutually exclusive; in this regard, the data that allowed formulation of a particular model did not exclude other possibilities. In addition, the types of stem and progenitor cells that arise in mice and humans may not be identical. As noted, despite an extensive literature describing the preferential prenatal development of B-1 B cells in mice, fetal B-1 development in humans has not been demonstrated, and whether stem cell independent yolk sac lymphopoiesis occurs is unclear. So, while the molecular layering model may not explain all of the cell types that arise during mouse fetal development, it may be sufficient to do so in humans.Many of the mutations that underlie various hematopoietic malignancies arise in utero, raising the question: do the properties of fetal progenitors, such as high proliferation rates and distinct patterns of gene expression predispose to the development and progression of particular leukemias? The review from Mendoza-Castrejon and Magee33 presents a comprehensive analysis of how layered immunity may instruct cell fates that underlie leukemogenicity. As those authors note, “if we can identify mechanisms that connect layered immunity to layered leukemogenicity, we can potentially identify age-specific therapeutic vulnerabilities to treat pediatric leukemia patients.” This review is noteworthy in that it presents a detailed discussion of leukemogenic mutations and how these may trigger leukemia at selective ages.It is now evident that distinct differences between fetal and adult hematopoiesis exist and that the emergence of different immune effectors occurs in waves. However, there is still much to be learned before consensual models, which may differ between species, can be formulated. How many waves of hematopoietic development exist? Which stem and progenitor cells function only transiently in the fetus and neonate and which are maintained long-term? Further studies that increase the understanding of how steady state adult hematopoiesis is sustained are also needed. One of the challenges in reconciling existing data is that different experimental approaches, as well as an inconsistent terminology when defining waves, were used, and some studies focused on mice while others utilized human cells. Furthermore, the results from lineage tracing studies are not always easy to interpret. Extensive discussion and collaborations between laboratories will be important as the field moves forward, and the editors hope the issues raised in this issue of Immunological Reviews will stimulate such interactions.The authors declare no conflicts of interest.","PeriodicalId":178,"journal":{"name":"Immunological Reviews","volume":"315 1","pages":"5-10"},"PeriodicalIF":7.5000,"publicationDate":"2023-03-24","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://onlinelibrary.wiley.com/doi/epdf/10.1111/imr.13198","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Immunological Reviews","FirstCategoryId":"3","ListUrlMain":"https://onlinelibrary.wiley.com/doi/10.1111/imr.13198","RegionNum":2,"RegionCategory":"医学","ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"Q1","JCRName":"IMMUNOLOGY","Score":null,"Total":0}

引用次数: 0

Abstract

It is fitting to begin the introduction to this volume of Immunological Reviews by discussing a 1986 review in this journal from Herzenberg and colleagues which introduced the concept of layered immune system development.¹ That contribution summarized functional differences between conventional B cells, which participate in adaptive immune responses and constitute the majority of B lymphocytes in mouse tissues, and a minor population of Ly-1 B cells that are innate-like effectors. Ly-1 B cells are now referred to as B-1 B cells while conventional B cells are designated as B-2 B cells. Based on data showing that neonatal bone marrow cells reconstituted B-1 B cells in irradiated recipients but adult bone marrow could not do so, B-1 and B-2 B cells were proposed to be distinct developmental lineages. This view was later reinforced by data from Hardy and Hayakawa, who discovered B-1 B cells in Leonore Herzenberg's laboratory,² showing that fetal liver pro-B cells could reconstitute cells with a B-1 B cell phenotype in immunodeficient mice while adult bone marrow cells failed to do so.³

The developmental distinctions between B-1 and B-2 B cells were the basis for a now widely cited 1989 commentary in Cell by Leonore and Leonard Herzenberg in which they presented the basic tenets of layered immune system development.⁴ Their layered immune system hypothesis proposed that the various types of lymphocytes that constitute the adult immune system developed in waves from distinct progenitors that emerged at different times during development. B-1 B cells emerged in the first, most primitive wave of development along with fetal erythrocytes and selected γδ T cells. A subsequent wave produced the so-called Ly-1 B sister population. The B-1 B cells in these two waves would now be referred to as B-1a and B-1b B cells which are known to function differently.^5-7 A third wave generated conventional B and T cells from self-replenishing progenitors in postnatal bone marrow throughout life. Studies conducted over the past 30 years have validated many aspects of the layered immune system hypothesis and suggested that the layering of immune system development is more extensive than initially envisioned by the Herzenbergs. The contributions that form this edition of Immunological Reviews provide a comprehensive summary of the evidence for developmental layering of many if not all lineages of the innate and adaptive immune system.

There is no general consensus regarding the number of waves of immune and hematopoietic system development that occur in the fetus and adult. However, the emergence of hematopoietic stem cells (HSCs) and lymphoid and myeloid progenitors in mice can be considered in the context of three broad developmental windows.

1. Pre HSC hematopoiesis: It has been recognized for decades that the extra-embryonic yolk sac is a site of early hematopoiesis and that red blood cells develop in that tissue prior to the emergence of HSCs,^{8, 9} which in the mouse occurs at embryonic day (E) 10.5. However, progenitors with myeloid potential also arise in the early yolk sac, and it is now established that their macrophage progeny are retained long-term in the adult as brain microglia, liver Kupffer cells, skin Langerhans cells, and alveolar macrophages.^{10, 11} The erythro-myeloid progenitors (EMPs) that arise as early as E8.25 in the yolk sac also generate mast cells, some of which are maintained in the adult. The contributions from Kobayashi and Yoshimoto¹² and from Chia et al.¹³ address the origin of mast cell progenitors during this early wave of yolk sac hematopoiesis as well as at later stages of development. In addition to discussing the origins of mast cells in different waves of hematopoiesis, the comprehensive chapter from Chia et al. reviews the impact of mast cells on various developmental and pathologic processes. Their review is a must read for those interested in mast cell biology. The Herzenberg's 1989 perspective⁴ proposed that many perplexing aspects of myeloid development can be clarified when viewed from the perspective of layered hematopoietic development, and the information contained in these reviews indicates they were correct.

Additional studies in mice surprisingly revealed that in addition to erythroid and myeloid cells, progenitors in the pre-HSC yolk sac can generate αβ and γδ T cells and B-1, but not B-2, B cells. Many of these revelations were initially made by Momoko Yoshimoto in collaboration with Mervyn Yoder and subsequently in her own independent laboratory and are summarized in the review by Kobayashi and Yoshimoto.¹² The degree to which B and T cells derived from this initial wave of lymphopoiesis contribute to fetal and/or adult immunity remain to be determined.

2. Mid-gestation hematopoiesis: Multiple hematopoietic populations are present in the mid-gestation fetus as discussed by Soares-da-Silva et al.¹⁴ and other reviews herein. These include HSCs, thymus seeding progenitors, B-1 and B-2 progenitors, and innate lymphoid progenitors (ILCs). The possibility that ILCs, and those in the ILC3 family in particular, emerge in separable waves of development are discussed in detail in the chapter from Van de Pavert¹⁵

It is not always easy to define the origin of the various progenitors present in the mid-gestation fetus, as some may have been generated in the pre-HSC period described above while others are likely the progeny of HSCs that emerge from hemogenic endothelium during this mid-gestation period. Further complicating the picture are recent studies concluding multi-potential progenitors (MPPs) arise from hemogenic endothelium in a wave(s) of development distinct from that of HSCs.^{16, 17} A major challenge will be to resolve the number of waves of lymphoid and myeloid development that arise within narrow time frames during mid-gestation and catalog the various stem and progenitor populations that are produced. The reviews from Montecino-Rodriguez and Dorshkind¹⁸ and Soares-da-Silva et al.¹⁴ which define several distinct waves of B and T cell development are relevant in this regard.

3. Adult hematopoiesis: A distinguishing characteristic of this period is the production of conventional B and T cells, while the generation of various innate-like lymphocytes either does not occur or is highly attenuated. For example, although γδ T cells can be generated in the adult thymus, the production of those that utilize the Vγ3 family is restricted to fetal hematopoiesis. Furthermore, the potential of adult marrow stem and progenitor cells to produce B-1a B cells is limited as discussed in reviews from Montecino-Rodriquez and Dorshkind¹⁸ and Koybayashi and Yoshimoto.¹² The latter reviews discuss the controversy regarding postnatal B-1 B cell development in light of studies showing the potential of adult marrow to generate those cells. The issue is not whether B-1 B cells, and B-1a B cells in particular, can develop from precursors in adult marrow but the efficiency with which they do so, and those reviews make the point that B-1 output from adult precursors is significantly attenuated compared to fetal progenitors. It is tempting to speculate that the few B-1 B cells generated in adult marrow are the progeny of a few fetal stem and progenitor cells that survive long-term after birth.

It has been suggested that adult bone marrow hematopoiesis does not adhere to the canonical model of hematopoiesis, which proposes that HSCs at the head of the hematopoietic hierarchy are responsible for all adult blood cell production. Kobayashi and Yoshimoto¹² review recent results from their group and the Carmago laboratory¹⁶ indicating that the fetal derived MPPs that arise distinct from HSCs as discussed above are retained in adult bone marrow long-term and make a significant contribution to adult lymphopoiesis for up to 2 years after birth. These recent findings are interesting in view of earlier barcoding studies indicating that progenitors, and not HSCs, are responsible for most day to day blood cell production.^{19, 20} However, this model has been challenged.²¹ These observations indicate that additional studies are needed to clarify how steady state blood cell production in the adult is sustained.

The results discussed above were obtained from analysis of mice, but there is evidence that layering of immune system development also occurs in humans as presented in three reviews in this issue of Immunological Reviews. Sanchez et al.²² discuss single cell sequencing results that support the existence of several distinct functional waves of γδ T cell development in the human fetal thymus. They also review the role of Lin28b and additional intrinsic and extrinsic factors in driving the fetal γδ T cell receptor repertoire in human γδ thymocytes. The contribution from Tabilas et al.²³ reviews evidence that the functions of CD8 T cells in adults is linked to when they were produced. For example, CD8 T cells in neonatal mice have rapid innate-like functions and those in adult animals have slower adaptive characteristics. Their chapter provides an overview of single cell sequencing results which support the existence of distinct ontogenic populations of CD8 T cells in humans. Burt and McCune²⁴ present a detailed review that also supports the layered development of human CD8 as well as CD4 T cells.

However, whether the layering of immune system development in humans is as extensive as in mice is unclear. For example, it has been challenging to identify human B-1 B cell progenitors. Until it is possible to do so, whether these cells emerge in distinct waves, if at all, in humans remains to be determined. Sun et al.²⁵ discuss the difficulty in definitively fate-mapping lymphoid cells in humans back to their developmental origin. As a result, they point out that, despite suggestive literature, it is difficult to conclude that human yolk sac progenitors give rise to lymphocytes in an HSC independent manner as has been shown in mice.

In fact, studies of early human lympho-hematopoiesis are challenging, because it is not easy to obtain human fetal tissues, particularly at precisely timed stages of development as discussed by Burt and McCune.²⁴ In addition, they point out that the sophisticated lineage tracing models that have been used in mice, discussed in the various chapters herein and the review from Van de Parvet¹⁵ in particular, are not available. That is why various in vitro models, including the generation of HSCs and progenitors from embryonic or induced pluripotent stem cells and systems such as the artificial thymus organ (ATO) cultures^{26, 27} will be important for defining the developmental potential of fetal and adult derived stem and progenitor cells as further discussed by Sun et al..²⁵ The ATO model is a particularly powerful system as it generates the full range of human T differentiation, including production of mature CD4⁺ and CD8⁺ T cells, and allows comparisons of development from fetal and adult hematopoietic stem and progenitor cells (HSPCs). For example, in contrast to postnatal thymopoiesis, terminal deoxynucleotidyl transferase (TdT) expression is absent during T cell differentiation from pluripotent stem cells in ATOs, reflecting a previously reported property of fetal lymphopoiesis.²⁸

If multiple populations of stem and progenitor cells with distinct developmental potential arise in different waves of fetal and adult hematopoiesis, it is reasonable to assume that they will exhibit differences in gene expression. The review from Montecino-Rodriguez and Dorshkind¹⁸ discusses how the genetic regulation of mouse B and T cell development within and between waves of fetal and adult lymphopoiesis differs. There are multiple waves of murine thymopoiesis as discussed in detail by Soares-da-Silva et al.¹⁴, and MacNabb and Rothenberg²⁹ present a masterful review that compares the transcription factor networks involved in T cell differentiation in the fetal and adult mouse thymus. Their review is distinguished by an elegant genetic analysis of genome-wide transcription data that has become available in recent years. As noted above, the single cell human sequencing studies have also revealed differences in gene expression in waves of human γδ T cell development as discussed by Sanchez et al.²²

At least two models can be formulated to explain the layering of immune and hematopoietic system development (Figure 1). The “Multiple Stem/Progenitor Cell model” proposes that multiple types of stem and progenitor cells with distinct developmental potential arise in overlapping waves of development. For example, Beaudin et al. identified a transient fetal HSC with the potential to produce innate-like lymphocytes (eg B-1 B cells, Vγ3⁺ γδ T cells) distinct from adult HSCs which primarily produced conventional B and T cells.³⁰ Their data provide support for the Herzenberg's prediction that “several types of hematopoietic stem cells that have evolved sequentially and function at specified times during development” exist. It is interesting, particularly in view of the detailed discussion by Soares-da-Silva et al.¹⁴ about when stem cell expansion in the fetus occurs, that the fetal HSCs described by Beaudin et al. were more proliferative than adult stem cells.

An alternative “Molecular Layering model” is presented in the review from Burt and McCune.²⁴ Based on single cell sequencing of human cord blood HSPCs and T cells, those investigators concluded that the stem and progenitor cell pool in the fetus is relatively homogeneous and that, at least from the perspective of T cell development, “the transition from human fetal to adult T cell identity and function does not occur due to a switch between distinct fetal and adult lineages. Rather, recent evidence from single cell analysis suggests that during the latter half of fetal development a gradual, en masse progressive transition occurs at the level of hematopoietic stem-progenitor cells (HSPCs) which is reflected in their T cell progeny”. This model is consistent with results from a mouse study by Kristiansen et al.³¹ who used a cellular barcoding approach to track individual HSPCs in the fetus and adult and showed that stem cells in the fetus could generate innate-like B-1 and selected γδ T cells and this potential was lost in the adult. These differences were linked to the expression of the Lin28b RNA binding protein, which is expressed in fetal and downregulated in adult HSCs. Interestingly, re-expression of Lin28b in adult HSCs allowed them to now produce innate like B and T cells. These observations raise the question of what regulates changes in gene expression in a fetal HSPC as it takes up residence in the adult? One possibility, as discussed by Burt and McCune,²⁴ is that HSPCs possesses an internal clock that coordinates changes in gene expression over time. Alternatively, changes in the environments stem cells occupy may trigger changes in gene expression.

In some cases, it is possible to explain the existence of particular fetal progenitors with either model. For example, our group defined a murine B-1 B cell restricted progenitor which we discuss in detail in our review in this volume.³² These progenitors are primarily present in fetal tissues and only at very low levels in adult bone marrow.³² If the multiple stem/progenitor cell model is considered, B-1 progenitors could arise directly, such as in the early yolk sac or in the mid-gestation embryo, in a stem cell independent manner. They, along with B-2 B cells and various myeloid progenitors could also be the progeny of fetal MPPs or HSCs. From the perspective of the molecular layering model, B-1 progenitors could be the progeny of a homogenous population of fetal HSCs that express Lin28b. However, as the expression of Lin28b and other fetal lineage specifying genes is downregulated, stem cells no longer generate B-1 and other innate-like progenitors or do so with significantly reduced efficiency. However, in other cases only the multiple stem/progenitor model can explain experimental results. For example, if distinct populations of HSCs and MPPs that arise independent from one another exist, their origin is difficult to explain based on the molecular layering model.

When attempting to reconcile data, it is important to consider that the two models are not mutually exclusive; in this regard, the data that allowed formulation of a particular model did not exclude other possibilities. In addition, the types of stem and progenitor cells that arise in mice and humans may not be identical. As noted, despite an extensive literature describing the preferential prenatal development of B-1 B cells in mice, fetal B-1 development in humans has not been demonstrated, and whether stem cell independent yolk sac lymphopoiesis occurs is unclear. So, while the molecular layering model may not explain all of the cell types that arise during mouse fetal development, it may be sufficient to do so in humans.

Many of the mutations that underlie various hematopoietic malignancies arise in utero, raising the question: do the properties of fetal progenitors, such as high proliferation rates and distinct patterns of gene expression predispose to the development and progression of particular leukemias? The review from Mendoza-Castrejon and Magee³³ presents a comprehensive analysis of how layered immunity may instruct cell fates that underlie leukemogenicity. As those authors note, “if we can identify mechanisms that connect layered immunity to layered leukemogenicity, we can potentially identify age-specific therapeutic vulnerabilities to treat pediatric leukemia patients.” This review is noteworthy in that it presents a detailed discussion of leukemogenic mutations and how these may trigger leukemia at selective ages.

It is now evident that distinct differences between fetal and adult hematopoiesis exist and that the emergence of different immune effectors occurs in waves. However, there is still much to be learned before consensual models, which may differ between species, can be formulated. How many waves of hematopoietic development exist? Which stem and progenitor cells function only transiently in the fetus and neonate and which are maintained long-term? Further studies that increase the understanding of how steady state adult hematopoiesis is sustained are also needed. One of the challenges in reconciling existing data is that different experimental approaches, as well as an inconsistent terminology when defining waves, were used, and some studies focused on mice while others utilized human cells. Furthermore, the results from lineage tracing studies are not always easy to interpret. Extensive discussion and collaborations between laboratories will be important as the field moves forward, and the editors hope the issues raised in this issue of Immunological Reviews will stimulate such interactions.

The authors declare no conflicts of interest.

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小鼠和人类分层免疫系统的发育

从1986年Herzenberg及其同事在《免疫学评论》杂志上发表的一篇综述开始介绍本卷是合适的，该综述介绍了分层免疫系统发育的概念这一贡献总结了传统B细胞和Ly-1 B细胞之间的功能差异。传统B细胞参与适应性免疫反应，构成小鼠组织中大部分B淋巴细胞，而Ly-1 B细胞是先天的效应细胞。Ly-1 B细胞现在被称为B-1 B细胞，而传统的B细胞被称为B-2 B细胞。根据数据显示，新生儿骨髓细胞在辐照受体中重建了B-1 B细胞，而成人骨髓不能重建B-1 B细胞，因此B-1和B-2 B细胞被认为是不同的发育谱系。这一观点后来被Hardy和Hayakawa的数据所证实，他们在Leonore Herzenberg的实验室中发现了B- 1b细胞，2表明胎儿肝前B细胞可以在免疫缺陷小鼠中重建具有B- 1b细胞表型的细胞，而成年骨髓细胞却不能。B-1和B-2细胞之间的发育差异是1989年Leonore和Leonard Herzenberg在《细胞》杂志上发表的一篇被广泛引用的评论的基础，他们在其中提出了分层免疫系统发育的基本原则他们的分层免疫系统假说提出，构成成人免疫系统的各种类型的淋巴细胞是在发育过程中不同时间出现的不同祖细胞的波状发育而成的。B-1 B细胞与胎儿红细胞和精选的γδ T细胞一起出现在发育的第一个最原始的波。随后的一波产生了所谓的ly - 1b姐妹种群。这两个波中的B-1 B细胞现在被称为B-1a和B-1b B细胞，它们的功能不同。第三波在出生后的骨髓中通过自我补充祖细胞产生常规的B细胞和T细胞。过去30年进行的研究已经证实了分层免疫系统假说的许多方面，并表明免疫系统发育的分层比herzenberg最初设想的更广泛。本期《免疫学评论》提供了许多(如果不是全部的话)先天和适应性免疫系统谱系发育分层证据的综合总结。关于免疫和造血系统发育在胎儿和成人中发生的波数没有普遍的共识。然而，小鼠造血干细胞(hsc)、淋巴祖细胞和髓祖细胞的出现可以在三个广泛的发育窗口的背景下考虑。造血干细胞形成前:几十年来，人们已经认识到胚胎外卵黄囊是早期造血的一个部位，红细胞在造血干细胞出现之前在该组织中发育8,9，在小鼠胚胎日(E) 10.5。然而，具有髓样潜能的祖细胞也出现在早期卵黄囊中，现在已经确定它们的巨噬细胞后代在成人中长期保留，如脑小胶质细胞、肝库普弗细胞、皮肤朗格汉斯细胞和肺泡巨噬细胞。10,11早在E8.25卵黄囊中出现的红髓祖细胞(EMPs)也产生肥大细胞，其中一些在成人中保持。Kobayashi和Yoshimoto12以及Chia等人13的贡献阐述了在卵黄囊造血的早期浪潮以及发育的后期阶段肥大细胞祖细胞的起源。除了讨论肥大细胞在不同造血过程中的起源外，Chia等人的综合章节还回顾了肥大细胞对各种发育和病理过程的影响。对于那些对肥大细胞生物学感兴趣的人来说，他们的评论是必读的。Herzenberg 1989年的观点4提出，从分层造血发育的角度来看，髓细胞发育的许多令人困惑的方面可以得到澄清，这些评论中包含的信息表明他们是正确的。对小鼠的进一步研究令人惊讶地发现，除了红细胞和髓细胞外，前hsc卵黄囊中的祖细胞可以产生αβ和γδ T细胞和B-1，但不能产生B-2 B细胞。许多这些发现最初是由Momoko Yoshimoto与Mervyn Yoder合作发现的，随后在她自己的独立实验室中进行，并在Kobayashi和Yoshimoto的综述中进行了总结。来自这一初始淋巴生成波的B细胞和T细胞对胎儿和/或成人免疫的贡献程度仍有待确定。妊娠中期造血:正如Soares-da-Silva等人14和本文其他综述所讨论的那样，妊娠中期胎儿中存在多个造血群体。这些细胞包括造血干细胞、胸腺种子祖细胞、B-1和B-2祖细胞以及先天淋巴样祖细胞(ILCs)。在Van de pavert15的章节中详细讨论了ilc，特别是ILC3家族中的ilc，在可分离的发育波中出现的可能性。定义妊娠中期胎儿中存在的各种祖细胞的起源并不总是容易的，因为有些可能在上述前hsc时期产生，而其他可能是在妊娠中期从造血内皮中产生的hsc的后代。更复杂的是，最近的研究得出结论，多潜能祖细胞(mpp)是由造血内皮形成的，其发育过程与造血干细胞不同。16,17一个主要的挑战将是解决在妊娠中期狭窄的时间框架内出现的淋巴细胞和髓细胞发育波的数量，并对产生的各种干细胞和祖细胞群体进行分类。Montecino-Rodriguez和Dorshkind18以及Soares-da-Silva等人14的综述定义了B细胞和T细胞发育的几个不同波，这与此相关。成人造血:这一时期的一个显著特征是常规B细胞和T细胞的产生，而各种先天样淋巴细胞的产生要么不发生，要么高度减弱。例如，虽然γδ T细胞可以在成人胸腺中产生，但利用Vγ3家族的细胞的产生仅限于胎儿造血。此外，成体骨髓干细胞和祖细胞产生B-1a B细胞的潜力是有限的，正如Montecino-Rodriquez和Dorshkind18以及Koybayashi和yoshimoto的综述所讨论的那样。后者的综述根据显示成体骨髓产生这些细胞的潜力的研究讨论了关于出生后B-1 B细胞发育的争议。问题不在于B-1 B细胞，特别是B-1a B细胞能否从成人骨髓的前体发育而来，而在于它们发育的效率。这些综述表明，与胎儿祖细胞相比，成人前体的B-1输出明显减弱。我们很容易推测，在成人骨髓中产生的少数B-1 B细胞是少数在出生后长期存活的胎儿干细胞和祖细胞的后代。有研究表明，成人骨髓造血并不遵循造血的规范模型，即造血系统中最高级的造血干细胞负责所有成人血细胞的产生。Kobayashi和Yoshimoto12回顾了他们的研究小组和Carmago实验室最近的研究结果，表明上述不同于造血干细胞的胎源性mpp长期保留在成人骨髓中，并在出生后长达2年的时间里对成人淋巴系统的形成做出了重大贡献。这些最近的发现很有趣，因为早期的条形码研究表明，祖细胞而不是造血干细胞负责大多数日常血细胞的产生。然而，这种模式受到了挑战这些观察结果表明，需要进一步的研究来阐明成年人的稳态血细胞生成是如何维持的。以上讨论的结果是通过对小鼠的分析得出的，但有证据表明免疫系统发育的分层也发生在人类身上，正如本期《免疫学评论》的三篇综述所述。Sanchez等人22讨论了单细胞测序结果，这些结果支持人类胎儿胸腺中存在几种不同的γδ T细胞发育功能波。他们还回顾了Lin28b和其他内在和外在因素在驱动人γδ胸腺细胞中胎儿γδ T细胞受体库中的作用。Tabilas等人23的贡献回顾了成人CD8 T细胞的功能与其产生时间有关的证据。例如，新生小鼠的CD8 T细胞具有快速的先天样功能，而成年动物的CD8 T细胞具有较慢的适应特征。他们的章节提供了单细胞测序结果的概述，这些结果支持人类中存在不同的CD8 T细胞个体群体。Burt和McCune24发表了一篇详细的综述，也支持人类CD8和CD4 T细胞的分层发育。然而，人类免疫系统发育的分层是否与小鼠一样广泛尚不清楚。例如，鉴定人类B- 1b B细胞祖细胞一直具有挑战性。在有可能做到这一点之前，这些细胞是否会以不同的波出现，如果有的话，在人类身上仍有待确定。Sun等人25讨论了确定人类淋巴样细胞命运定位到其发育起源的困难。因此，他们指出，尽管有暗示性的文献，但很难得出人类卵黄囊祖细胞以独立于HSC的方式产生淋巴细胞的结论，正如在小鼠中所显示的那样。事实上，早期人类淋巴造血的研究是具有挑战性的，因为获取人类胎儿组织并不容易，特别是在Burt和mccune所讨论的精确的发育阶段此外，他们还指出，在本文的各个章节以及Van de Parvet15的评论中讨论的用于小鼠的复杂的谱系追踪模型是不可用的。这就是为什么各种体外模型，包括从胚胎或诱导多能干细胞和系统(如人工胸腺器官(ATO)培养26,27)中产生造血干细胞和祖细胞，对于定义胎儿和成人衍生干细胞和祖细胞的发育潜力非常重要，Sun等人进一步讨论了这一点ATO模型是一个特别强大的系统，因为它可以产生全方位的人类T细胞分化，包括成熟CD4+和CD8+ T细胞的产生，并允许比较胎儿和成人造血干细胞和祖细胞(HSPCs)的发育。例如，与出生后的胸腺生成相反，ATOs中多能干细胞向T细胞分化的过程中不存在末端脱氧核苷酸转移酶(TdT)表达，这反映了先前报道的胎儿淋巴生成的特性。如果在胎儿和成人造血的不同阶段产生具有不同发育潜力的多个干细胞和祖细胞群体，我们有理由认为它们在基因表达上存在差异。Montecino-Rodriguez和Dorshkind18的综述讨论了小鼠B细胞和T细胞发育的遗传调控在胎儿和成人淋巴生成周期内和之间的差异。Soares-da-Silva等人详细讨论了小鼠胸腺发育的多个波14,MacNabb和Rothenberg29对胎儿和成年小鼠胸腺中参与T细胞分化的转录因子网络进行了比较。他们的综述的特点是对近年来可用的全基因组转录数据进行了优雅的遗传分析。如上所述，单细胞人类测序研究也揭示了人类γδ T细胞发育波中基因表达的差异，如Sanchez等人所讨论的那样22至少可以制定两种模型来解释免疫和造血系统发育的分层(图1)。“多干细胞/祖细胞模型”提出，在重叠的发育波中出现了具有不同发育潜力的多种类型的干细胞和祖细胞。例如，Beaudin等人发现一种瞬时的胎儿造血干细胞具有产生先天样淋巴细胞(如B-1 B细胞，Vγ3+ γδ T细胞)的潜力，而成人造血干细胞主要产生传统的B细胞和T细胞他们的数据为Herzenberg的预测提供了支持，即“几种类型的造血干细胞在发育过程中按顺序进化并在特定时间起作用”。有趣的是，特别是考虑到Soares-da-Silva等人14关于干细胞在胎儿中何时发生扩增的详细讨论，Beaudin等人描述的胎儿造血干细胞比成体干细胞更具增殖性。Burt和mccune的综述中提出了另一种“分子分层模型”基于人类脐带血HSPCs和T细胞的单细胞测序，这些研究人员得出结论，胎儿的干细胞和祖细胞池相对均匀，至少从T细胞发育的角度来看，“从人类胎儿到成人T细胞的身份和功能的转变并不是因为在不同的胎儿和成人谱系之间的转换而发生的。”相反，最近来自单细胞分析的证据表明，在胎儿发育的后半期，造血干细胞(HSPCs)水平发生了逐渐的、整体的渐进式转变，这反映在它们的T细胞后代中。”该模型与Kristiansen等人的小鼠研究结果一致，他们使用细胞条形码方法跟踪胎儿和成人中的单个HSPCs，结果表明胎儿中的干细胞可以产生先天样的B-1和选择性γδ T细胞，而这种潜力在成人中丢失。这些差异与Lin28b RNA结合蛋白的表达有关，该蛋白在胎儿中表达，在成人造血干细胞中下调。有趣的是，Lin28b在成人造血干细胞中的重新表达使它们现在能够产生先天的B细胞和T细胞。这些观察结果提出了一个问题:当胎儿HSPC在成人中定居时，是什么调节了基因表达的变化?正如Burt和McCune所讨论的那样，一种可能性是HSPCs拥有一个内部时钟，可以随着时间的推移协调基因表达的变化。或者，干细胞所处环境的变化可能引发基因表达的变化。在某些情况下，用任何一种模型都可以解释特定胎儿祖先的存在。例如，我们小组定义了一种小鼠B-1 B细胞限制性祖细胞，我们将在本卷的综述中详细讨论这些祖细胞主要存在于胎儿组织中，仅在成人骨髓中含量极低如果考虑多干/祖细胞模型，B-1祖细胞可以直接产生，例如在早期卵黄囊或妊娠中期胚胎中，以干细胞独立的方式产生。它们，连同B-2 B细胞和各种髓系祖细胞也可能是胎儿MPPs或造血干细胞的后代。从分子分层模型的角度来看，B-1祖细胞可能是表达Lin28b的同质胎hsc群体的后代。然而，随着Lin28b和其他胎儿谱系指定基因的表达下调，干细胞不再产生B-1和其他先天样祖细胞或产生效率显著降低。然而，在其他情况下，只有多干/祖模型可以解释实验结果。例如，如果存在彼此独立产生的hsc和mpp的不同种群，则很难根据分子分层模型解释它们的起源。当试图调和数据时，重要的是要考虑到这两个模型不是相互排斥的;在这方面，允许制定特定模型的数据并不排除其他可能性。此外，小鼠和人类体内产生的干细胞和祖细胞的类型可能不相同。如上所述，尽管大量文献描述了B-1 B细胞在小鼠中的优先产前发育，但胎儿B-1在人类中的发育尚未得到证实，并且干细胞独立卵黄囊淋巴形成是否发生尚不清楚。因此，虽然分子分层模型可能无法解释小鼠胎儿发育过程中出现的所有细胞类型，但它可能足以解释人类。许多导致各种造血恶性肿瘤的突变都是在子宫内发生的，这就提出了一个问题:胎儿祖细胞的特性，如高增殖率和不同的基因表达模式，是否易导致特定白血病的发生和进展?Mendoza-Castrejon和Magee33的综述全面分析了分层免疫如何指导导致白血病发生的细胞命运。正如这些作者所指出的那样，“如果我们能够确定将分层免疫与分层白血病发生性联系起来的机制，我们就有可能确定治疗儿科白血病患者的年龄特异性治疗脆弱性。”这篇综述值得注意的是，它提出了白血病发生突变的详细讨论，以及这些突变如何在选择性年龄引发白血病。现在很明显，胎儿和成人造血存在明显差异，不同免疫效应器的出现是分波发生的。然而，在形成可能因物种而异的共识模型之前，仍有许多东西需要学习。有多少波造血发育存在?哪些干细胞和祖细胞在胎儿和新生儿中只起短暂作用，哪些是长期维持的?还需要进一步的研究来增加对成人稳态造血如何维持的理解。调和现有数据的挑战之一是使用了不同的实验方法，以及在定义波时使用了不一致的术语，并且一些研究侧重于小鼠，而另一些研究则使用了人类细胞。此外，谱系追踪研究的结果并不总是容易解释。随着该领域的发展，实验室之间的广泛讨论和合作将是重要的，编辑们希望本期《免疫学评论》提出的问题将刺激这种互动。作者声明无利益冲突。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Immunological Reviews 医学-免疫学

CiteScore

16.20

自引率

1.10%

发文量

118

审稿时长

4-8 weeks

期刊介绍： Immunological Reviews is a specialized journal that focuses on various aspects of immunological research. It encompasses a wide range of topics, such as clinical immunology, experimental immunology, and investigations related to allergy and the immune system. The journal follows a unique approach where each volume is dedicated solely to a specific area of immunological research. However, collectively, these volumes aim to offer an extensive and up-to-date overview of the latest advancements in basic immunology and their practical implications in clinical settings.