Difference between revisions of "Part:BBa K1189024"

(Contribution (Waterloo iGEM 2020))
(Contribution (Waterloo iGEM 2020))
 
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Stability:
 
Stability:
- In vitro, H ferritin oxidizes iron at a much faster rate than L ferritin because of the presence of a particular ferroxidase centre in H ferritin that is absent in L ferritin (Santambrogio et al., 1993)
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* In vitro, H ferritin oxidizes iron at a much faster rate than L ferritin because of the presence of a particular ferroxidase centre in H ferritin that is absent in L ferritin (Santambrogio et al., 1993)
- L ferritin induces iron mineralization more efficiently than H ferritin (Santambrogio et al., 1993)
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* L ferritin induces iron mineralization more efficiently than H ferritin (Santambrogio et al., 1993)
- L ferritin is able to withstand physical denaturation better than H ferritin because of the replacement of the ferroxidase centre of the H chain with a salt bridge in the L-chain (Santambrogio et al., 1993)
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* L ferritin is able to withstand physical denaturation better than H ferritin because of the replacement of the ferroxidase centre of the H chain with a salt bridge in the L-chain (Santambrogio et al., 1993)
  
 
'''References''':
 
'''References''':
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Santambrogio, P. et al. (1993). Production and Characterization of Recombinant Heteropolymers of Human Ferritin H and L Chains. ''The Journal of Biological Chemistry, 268''(17). 12744-12748.
 
Santambrogio, P. et al. (1993). Production and Characterization of Recombinant Heteropolymers of Human Ferritin H and L Chains. ''The Journal of Biological Chemistry, 268''(17). 12744-12748.
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<!-- Add more about the biology of this part here
 
<!-- Add more about the biology of this part here

Latest revision as of 02:09, 21 October 2020

Light chain human ferritin

This part is the light ferritin subunit from human ferritin, inspired by P02792 [UniParc]. Ferritin is ubiquitous across prokaryotic and eukaryotic systems and is used to buffer intracellular iron. This part, along with the heavy ferritin subunit, form a 24 multimeric iron sequestering nanoparticle (Chasteen et al., 1991). The light ferritin purportedly contributes to nucleation to initiate iron core formation in ferritin molecules (Chasteen et al., 1999). These nanoparticles are robust, remain stable at extreme pHs, and withstand temperature variations (Kim et al., 1999).

Ferritin

Figure 1. Ribbon visualization of a fully assembled ferritin protein.

Ferritin's utility in iGEM

Ferritin as a nanoparticle is interesting for other iGEM teams for two reasons. Firstly, its iron core can be replaced with other compounds to serve different functions. The iGEM Calgary 2013 demonstrated this by chemically modifying recombinant ferritin's iron core into a robust colourmetric reporter. Other intriguing applications include making ferritin’s iron core magnetically active as magnetoferritin (Jordan et al. 2013), using ferritin as a nanocage for other metals, or the incorporation of other reporters such as quantum dots (Naito et al. 2013) (Figure 2).

Ferritin Core Modulation

Figure 2. Chemically modifying the iron core of ferritin allows ferritin to be moulded to fit a wide magnitude of applications. Additionally the ferritin subunits can act as a nanocage to encapsulate completely new cores.

Secondly, the ferritin nanoparticle is useful for iGEM teams as a self-assembling and spherical protein scaffold. Each of the 24 subunits forming ferritin can be fused to proteins of interest, such that when the nanoparticle assembles, proteins surround the ferritin sphere (Kim et al., 2011). The iGEM Calgary 2013 team demonstrated this by binding DNA sensing proteins, TALEs, as part of their FerriTALE sensor. The Calgary team also constructed ferritin subunits with a coiled-coil linker system so that other teams can scaffold proteins to E-coil ferritin (BBa_K1189018, BBa_K1189019, BBa_K1189020, BBa_K1189037). See Figure 3 for a demonstration of these applications.

FerriTALE Scaffold Modularity

Figure 3. Using the E and K coils in combination with ferritin as a scaffold system allows the creation of brand new FerriTALEs or protein scaffolds.

References

  • Chasteen, N. D., & Harrison, P. M. (1999). Mineralization in ferritin: an efficient means of iron storage. Journal of structural biology, 126(3), 182-194.
  • Clavijo Jordan, V., Caplan, M. R., & Bennett, K. M. (2010). Simplified synthesis and relaxometry of magnetoferritin for magnetic resonance imaging. Magnetic Resonance in Medicine, 64(5), 1260-1266.
  • Kim, S. E., Ahn, K. Y., Park, J. S., Kim, K. R., Lee, K. E., Han, S. S., & Lee, J. (2011). Fluorescent ferritin nanoparticles and application to the aptamer sensor. Analytical chemistry, 83(15), 5834-5843.
  • Naito, M., Iwahori, K., Miura, A., Yamane, M., & Yamashita, I. (2010). Circularly polarized luminescent CdS quantum dots prepared in a protein nanocage. Angewandte Chemie International Edition, 49(39), 7006-7009.


  • Contribution (Waterloo iGEM 2020)

    Summary: While the heavy and light chain human ferritin subunits have been added to the iGEM parts registry with adequate description of their function, we wanted to compare them more thoroughly. Therefore, our discussion includes both chains’ stability and ability to uptake iron.

    Documentation: Human ferritin heteropolymers can be composed with varying ratios of heavy (H) and light (L) chains, and different forms exist naturally depending on the tissue examined (Boyd et al., 1985). However, the knowledge of the two chains is not sufficient enough to predict the properties of any given heteropolymer.

    Homopolymers composed of strictly light or heavy chains can be synthesized, which can be advantageous as heavy and light chains have different properties: 1. H-rich ferritins turn over more rapidly than L-rich ferritins 2. H-rich ferritins accumulate in iron-rich tissues 3. L-rich ferritins take up and release iron more rapidly than L-rich ferritins

    Within the shell, H and L subunits are interchangeable as the key residues are conserved.

    L subunits contain 15 hydrophilic iron binding residues, while only 7 of these exist in H subunits. This results in a reduced ability to nucleate iron in H subunits, causing faster iron uptake and release as well as less iron accumulation in H-rich ferritins.

    Ferritin’s uptake of iron is either driven by H-chain ferroxidase activity (Levi et al., 1988) or driven by iron autoxidation which occurs in the absence of H-chains.

    Stability:

    • In vitro, H ferritin oxidizes iron at a much faster rate than L ferritin because of the presence of a particular ferroxidase centre in H ferritin that is absent in L ferritin (Santambrogio et al., 1993)
    • L ferritin induces iron mineralization more efficiently than H ferritin (Santambrogio et al., 1993)
    • L ferritin is able to withstand physical denaturation better than H ferritin because of the replacement of the ferroxidase centre of the H chain with a salt bridge in the L-chain (Santambrogio et al., 1993)

    References:

    Boyd, D., Vecoli, C., Belcher, D.M., Jain, S.W., & Drysdale, J.W. (1985). Structural and Functional Relationships of Human Ferritin H and L Chains Deduced from cDNA Clones. The Journal of Biological Chemistry, 260(21). 11755-11761.

    Levi, S. et al. (1988). Mechanism of Ferritin Iron Uptake: Activity of the H-chain and Deletion Mapping of the Ferro-oxidase Site. The Journal of Biological Activity, 263(34). 18086-18092.

    Santambrogio, P. et al. (1993). Production and Characterization of Recombinant Heteropolymers of Human Ferritin H and L Chains. The Journal of Biological Chemistry, 268(17). 12744-12748.



    Sequence and Features


    Assembly Compatibility:
    • 10
      COMPATIBLE WITH RFC[10]
    • 12
      COMPATIBLE WITH RFC[12]
    • 21
      COMPATIBLE WITH RFC[21]
    • 23
      COMPATIBLE WITH RFC[23]
    • 25
      COMPATIBLE WITH RFC[25]
    • 1000
      INCOMPATIBLE WITH RFC[1000]
      Illegal BsaI.rc site found at 391