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Hematopoietic stem cell - Wikipedia, the free encyclopedia

Hematopoietic stem cell

From Wikipedia, the free encyclopedia

Note that some complexity is omitted from the diagram. Lymphocytes come from "Lymphoid" line, while granulocytes, monocytes, megakaryocytes, and erythrocytes come from "Myeloid" line. Among myeloid cells, granulocytes and monocytes have a common precursor, "CFU-GM".
Note that some complexity is omitted from the diagram. Lymphocytes come from "Lymphoid" line, while granulocytes, monocytes, megakaryocytes, and erythrocytes come from "Myeloid" line. Among myeloid cells, granulocytes and monocytes have a common precursor, "CFU-GM".

Hematopoietic stem cells (HSC) are stem cells and the early precursor cells which give rise to all the blood cell types that include both the myeloid (monocytes and macrophages, neutrophils, basophils, eosinophils, erythrocytes, megakaryocytes/platelets and some dendritic cells) and lymphoid lineages (T-cells, B-cells, NK-cells, some dendritic cells). The definition of hematopoietic stem cells have undergone considerable revision in the last two decades. The hematopoietioc tissue have cells with long term and short term regeneration capacities and committed multipotent, oligopotent and unipotent progenitors.

Contents

[edit] Source

Sketch of bone marrow and its cells
Sketch of bone marrow and its cells

HSC are found in the bone marrow of adults, which includes femurs, hip, ribs, sternum, and other bones. Cells can be obtained directly by removal from the hip using a needle and syringe, or from the blood following pre-treatment with cytokines, such as G-CSF (granulocyte colony stimulating factors), that induce cells to be released from the bone marrow compartment. Other sources for clinical and scientific use include umbilical cord blood, placenta, molilized peripheral blood. For experimental purposes, fetal liver, fetal spleen and AGM (Aorta-gonad-mesonephros) of animals are also useful sources of HSCs.

[edit] Functional Characteristics

[edit] multipotency and self-renewal

As stem cells, they are defined by their ability to form multiple cell types (multipotency) and their ability to self-renew.

Multipotency: Individual HSC have the ability to give rise to any of the end-stage blood cell types. During differentiation, daughter cells derived from HSC undertake a series of commitment decisions, retaining differentiation potential for some lineages while losing others. Intermediate cells become progressively more restricted in their lineage potential, until eventually lineage-committed end stage cells are generated.

Self-Renewal: Some kinds of stem cells are thought to undertake asymmetric cell division, generating one daughter cell that remains a stem cell and one daughter cell that differentiates. For Hematopoietic Stem Cells, however, whether asymmetric cell division occurs during self-renewal is not known with certainty. It is instead possible that hematopoiesis occurs via symmetrical divisions, that sometimes give rise to two daughter HSC, and that at other times give rise to progeny that are committed to differentiate. The balance between self-renewal versus differentiation would therefore be regulated by the control of these two kinds of symmetrical cell division.

It is known that a small number of HSC can expand to generate a very large number of progeny HSC. This phenomenon is used in bone marrow transplant when a small number of HSC reconstitute the hematopoietic system. This indicates that at least during bone marrow transplant, symmetrical cell divisions that give two progeny HSC must occur, as expansion in HSC numbers seen during bone marrow transplant cannot occur in any other way.

Stem cell self-renewal is thought to occur in the stem cell niche in the bone marrow, and it is reasonable to assume that key signals present in this niche will be important in self-renewal. There is much interest in the environmental and molecular requirements for HSC self-renewal, as understanding the ability of HSC to replenish themselves will eventually allow the generation of expanded populations of HSC ex vivo that can be used therapeutically.

[edit] Functional Assays

  • Cobble stone area forming Cell (CFAC) assay: This is a cell culture based empirical assay. When plated onto a confluent culture of stromal feeder layer, a fraction of HSCs creep between the gaps (even though the stromal cells are touching each other) and eventually settle between the stromal cells and the substratum (here the dish surface) or trapped in the cellular processes between the stromal cells. Emperipolesis is the in vivo phenomenon in which one cell is completely engulfed into another (eg thymocytes into thymic nurse cells); on the other hand, when, in vitro, lymphoid lineage cells creep beneath nurse like cells it is called pseudoemperipolesis. This similar phenomeonon is more commonly known in HSC field by the cell culture terminology cobble stone area forming cells (CFAC) which means areas of cluster of cells which look dull cobblestone-like under phase contrast microscopy, compared to the other HSCs which are refractile. This happens because the cells which are folating loosely on top of the stromal cells are spherical and thus refractile. However, the cells which creep beneath the stromal cells are flattened and thus not refractile. The mechanism of pseudoemperipolesis is only recently coming to light. it may be mediated by interection through CXCR4 (CD184) the receptor for CXC Chemokines (eg SDF1) and α4β1 integrins.[1].

[edit] Physical characteristics

Hematopoietic stem cells morphologically resemble lymphocytes. They are non-adherent, rounded, rounded nucleus, and low cytoplasm to nucleus ratio. Since PHSC can not be isolated as a pure population, it is not possible to identify them in a microscope. The above description is based on the morphological characteristics of a heterogeneous population of which PHSC are a component.


[edit] Markers

Hematopoeitic stem cells are phenotypically identified by their small size, lack of lineage (lin) markers, low staining (side population) with vital dyes such as rhodamine 123 (rhodamineDULL, also called rholo) or Hoechst 33342, and presence of various antigenic markers on their surface many of which belongs to the cluster of differentiation series, like: CD34, CD38, CD90, CD133, CD105, CD45 and also c-kit- the receptor for stem cell factor. The hematopoietic stem cells are negative for the markers which are used for detection of lineage commitment and are thus called Lin-, and during their purification by FACS, a bunch of upto 13 to 14 different mature blood-lineage marker eg CD13 & CD33 for myeloid, CD71 for erythroid, CD19 for B cells, CD61 for megakaryocytic etc for humans; and, B220 (murine CD45) for B cells, Mac-1 (CD11b/CD18) for monocytes, Gr-1 for Granulocytes, Ter119 for erythroid cells, Il7Ra, CD3, CD4, CD5, CD8 for T cells etc for mice) antibodies are used as a mixture to deplete the lin+ cells or late multipotent progenitors (MPP)s.

There are a lot of differences between the human and mice hematopoietic cell markers for the commonly accepted type of hematopoietic stem cells.[1].

However not all stem cells are covered by these combinations which nonetheless have become pupular. In fact even in humans there are hematopoietic stem cells which are CD34-/CD38-. [2][3]. Also some later studies suggested that earliest stem cells may lack c-kit on the cell surface[4]. For human HSCs use of CD133 was one step ahead as both CD34+ and CD34- HSCs were CD133+.

Traditional purification method used to yield a reasonable purity level of mouse hematopoietic stem cells generally requires a large(~10-12) battery of markers, most of which were surrogate markers with little functional significance and thus partial overlap with the stem cell populations and sometimes other closely related cells which are not stem cells. Also some of these markers 9eg Thy1) are not conserved across mouse species, and use of markers like CD34- for HSC purification requires mice to be at least 8 weeks old. Alternative methods which could give rise to similar or better harvest of stem cells is a hot area of research and are presently emerging. One such method uses a signature of SLAM family of cell surface molecules. SLAM (Signaling lymphocyte activation molecule) family is a group of >10 molecules whose genes are mostly located tandemly in a single locus on chromosome 1 (mouse), all belonging to a subset of immunoglobulin gene superfamily, and originally thought to be involved in T-cell stimulation. This family includes CD48, CD150, CD244 etc, CD150 being the founding member thus also called slamF1 ie SLAM family member 1.

The signature SLAM code for the hemapoietic higherchy are:

  • Hematopoietic stem cells (HSC) : CD150+CD48-CD244-
  • Multipotent progenitor cells (MPPs) : CD150-CD48-CD244+
  • Lineage-restricted progenitor cells (LRPs) : CD150-CD48+CD244+

For HSCs CD150+CD48- was sufficient instead of CD150+CD48-CD244- because CD48 is a ligand for CD244 and both would be positive only in the activated lineage restricted progenitors. This code was more efficient than the more tedious earlier set of the large number of markers and are also conserved across the mouse strains.[5]. CD150+CD48- gave stem cell purity comparable to Thy1loSca-1+lin-c-kit+ in mice.[6]

Irving Weissman's group at Stanford University that was the first to isolate mouse hematopoietic stem cells in 1988, was also the first to work out the markers to distinguish the mouse long term (LT-HSC) and short term (ST-HSC) hematopoietic stem cells (self renew capable), and the Multipotent progenitors (MPP, low or no self renew capability — the later the developmental stage of MPP, the lesser the self renewal ability and the more of some of the markers like CD4 and CD135):

[edit] Nomenclature of hematopoietic colonies and lineages

Between 1948 and 1950, the Committee for Clarification of the Nomenclature of Cells and Diseases of the Blood and Blood-forming Organs issued reports on the nomenclature of blood cells.[7][8] An overview of the terminology is shown below, from earliest to final stage of development:

  • [root]blast
  • pro[root]cyte
  • [root]cyte
  • meta[root]cyte
  • mature cell name

The root for CFU-E is "rubri", for CFU-GM is "granulo" or "myelo" and "mono", for CFU-L is "lympho" and for CFU-Me is "megakaryo". According to this terminology, the stages of red blood cell formation would be: rubriblast, prorubricyte, rubricyte, metarubricyte and finally erythrocyte. However, the following nomenclature seems to be, at present, the most prevalent:

Committee "lympho" "rubri" "granulo" or "myelo" "mono" "megakaryo"
Lineage Lymphoid Myeloid Myeloid Myeloid Myeloid
CFU CFU-L CFU-E CFU-GM CFU-GM CFU-Me
Process lymphocytopoiesis erythropoiesis granulocytopoiesis monocytopoiesis thrombocytopoiesis
[root]blast Lymphoblast Proerythroblast Myeloblast Monoblast Megakaryoblast
pro[root]cyte Prolymphocyte Polychromatophilic erythrocyte Promyelocyte Promonocyte Promegakaryocyte
[root]cyte - Normoblast Eosino/neutro/basophilic myelocyte Megakaryocyte
meta[root]cyte Large lymphocyte Reticulocyte Eosinophilic/neutrophilic/basophilic metamyelocyte, Eosinophilic/neutrophilic/basophilic band cell Early monocyte -
mature cell name Small lymphocyte Erythrocyte granulocytes (Eosino/neutro/basophil) Monocyte thrombocytes (Platelets)

Osteoclasts also arise from haemopoietic cells of the monocyte/neutrophil lineage, specifically CFU-GM.

[edit] Colony-forming units

There are various kinds of colony-forming units:

The above CFUs are based on the lineage. Another CFU, the colony-forming unit–spleen (CFU–S) was the basis of an in vivo clonal colony formation, which depends on the ability of infused bone marrow cells to give rise to clones of maturing hematopoietic cells in the spleens of irradiated mice after 8 to 12 days. It was used extensively in early studies, but is now considered to measure more mature progenitor or Transit Amplifying Cells rather than stem cells.

[edit] References

  1. ^ Burger JA, Spoo A, Dwenger A, Burger M, Behringer D. CXCR4 chemokine receptors (CD184) and alpha4beta1 integrins mediate spontaneous migration of human CD34+ progenitors and acute myeloid leukaemia cells beneath marrow stromal cells (pseudoemperipolesis). Br J Haematol. 2003 Aug;122(4):579-89. PMID: 12899713
  2. ^ Bhatia, M., D. Bonnet, B. Murdoch, O.I. Gan and J.E. Dick, A newly discovered class of human hematopoietic cells with SCID-repopulating activity, 4(9), 1038, 1998.
  3. ^ Guo, Yalin , Lubbert, Michael , Engelhardt, Monika CD34- Hematopoietic Stem Cells: Current Concepts and Controversies Stem Cells 2003; 21: 15-20; First published online ; doi:10.1634/stemcells.21-1-15
  4. ^ H. Doi et al. (1997) Proc. Natl. Acad. Sci. USA 94, 2513–2517
  5. ^ Gary Van Zant Stem cell markers: less is more! Blood 107: 855-856.
  6. ^ Kiel et al, Cell, Vol. 121, 1109–1121, July 1, 2005, Copyright ©2005 by Elsevier Inc. DOI 10.1016/j.cell.2005.05.026
  7. ^ (1948) "First report of the Committee for Clarification of the Nomenclature of Cells and Diseases of the Blood and Blood-forming Organs.". Amer J Clin Pathol 18: 443-450. 
  8. ^ (1950) "Third, fourth and fifth reports of the committee for clarification of the nomenclature of cells and diseases of the blood and blood-forming organs.". Am J Clin Pathol 20 (6): 562-79. PMID 15432355. 

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