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词条 Phycobiliprotein
释义

  1. Major phycobiliproteins

  2. Characteristics and applications in biotechnology

  3. References

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Phycobiliproteins are water-soluble proteins present in cyanobacteria and certain algae (rhodophytes, cryptomonads, glaucocystophytes) which capture light energy, which is then passed on to chlorophylls during photosynthesis. Phycobiliproteins are formed of a complex between proteins and covalently bound phycobilins that act as chromophores (the light-capturing part). They are most important constituents of the phycobilisomes.

Major phycobiliproteins

Phycobiliprotein MW (kDa) Ex (nm) / Em (nm) Quantum yield Molar Extinction Coefficient (M−1cm−1) Comment Image
R-Phycoerythrin (R-PE) 240 498.546.566 nm / 576 nm 0,84 1.53 106 Can be excited by Kr/Ar laser
Applications for R-Phycoerythrin

Many applications and instruments were developed specifically for R-phycoerythrin. It is commonly used in immunoassays such as FACS, flow cytometry, multimer/tetramer applications.

Structural Characteristics

R-phycoerythrin is also produced by certain red algae. The protein is made up of at least three different subunits and varies according to the species of algae that produces it. The subunit structure of the most common R-PE is (αβ)6γ. The α subunit has two phycoerythrobilins (PEB), the β subunit has 2 or 3 PEBs and one phycourobilin (PUB), while the different gamma subunits are reported to have 3 PEB and 2 PUB (γ1) or 1 or 2 PEB and 1 PUB (γ2).

(Phycobiliprotein overview information)
B-Phycoerythrin (B-PE) 240 546.566 nm / 576 nm 0,98 (545 nm) 2.4 106

(563 nm) 2.33 106

Applications for B-Phycoerythrin

Because of its high quantum yield, B-PE is considered the world’s brightest fluorophore. It is compatible with commonly available lasers and gives exceptional results in flow cytometry, Luminex® and immunofluorescent staining. B-PE is also less “sticky” than common synthetic fluorophores and therefore gives less background interference.

Structural Characteristics

B-phycoerythrin (B-PE) is produced by certain red algae such as Rhodella sp. The specific spectral characteristics are a result of the composition of its subunits. B-PE is composed of at least three subunits and sometimes more. The chromophore distribution is as follows: α subunit with 2 phycoerythrobilins (PEB), β subunit with 3 PEB, and the γ subunit with 2 PEB and 2 phycourobilins (PUB). The quaternary structure is reported as (αβ)6γ.

(Phycobiliprotein overview information)
C-Phycocyanin (CPC) 232 620 nm / 642 nm 0,81 1.54 106 Accepts the fluorescence for R-PE; Its red fluorescence can be transmitted to Allophycocyanin
Allophycocyanin (APC) 105 651 nm / 662 nm 0,68 7.3 105 Excited by He/Ne laser; double labeling with Sulfo-Rhodamine 101 or any other equivalent fluorochrome.
Applications for Allophycocyanin

Many applications and instruments were developed specifically for allophycocyanin. It is commonly used in immunoassays such as flow cytometry and high-throughput screening. It is also a common acceptor dye for FRET assays.

Structural Characteristics

Allophycocyanin can be isolated from various species of red or blue-green algae, each producing slightly different forms of the molecule. It is composed of two different subunits (α and β) in which each subunit has one phycocyanobilin (PCB) chromophore. The subunit structure for APC has been determined as (αβ)3.

(Phycobiliprotein overview information)
↑ = FluoProbes PhycoBiliProteins data

Characteristics and applications in biotechnology

Phycobiliproteins elicit great fluorescent properties compared to small organic fluorophores, especially when high sensitivity or multicolor detection is required :

  • Broad and high absorption of light suits many light sources
  • Very intense emission of light: 10-20 times brighter than small organic fluorophores
  • Relative large Stokes shift gives low background, and allows multicolor detections.
  • Excitation and emission spectra do not overlap compared to conventional organic dyes.
  • Can be used in tandem (simultaneous use by FRET) with conventional chromophores (i.e. PE and FITC, or APC and SR101 with the same light source).
  • Fluorescence retention period is longer.
  • Very high water solubility

As a result, phycobiliproteins allow very high detection sensitivity, and can be used in various fluorescence based techniques [https://store-7fikt.mybigcommerce.com/product_images/uploaded_images/Telford_Cyanobacterial_stabilized_phycobilisomes-2001.pdf fluorimetric microplate assays],[6] [https://store-7fikt.mybigcommerce.com/product_images/uploaded_images/Telford_Cyanobacterial_stabilized_phycobilisomes-2001.pdf Flow Cytometry],[7] FISH and multicolor detection.

References

1. ^{{Cite journal |url=http://www.rcsb.org/pdb/explore/explore.do?structureId=1EYX |title=Crystal structure of R-phycoerythrin at 2.2 angstroms |author=Contreras-Martel, C. |display-authors=4 |author2=Legrand, P. |author3=Piras, C. |author4=Vernede, X. |author5=Martinez-Oyanedel, J. |author6=Bunster, M. |author7=Fontecilla-Camps, J.C. |date=2000-05-09 |publisher=RCSB Protein Data Bank (PDB) |id=PDB ID: 1EYX |doi=10.2210/pdb1eyx/pdb |access-date=11 October 2012}}
2. ^{{cite journal | vauthors = Contreras-Martel C, Martinez-Oyanedel J, Bunster M, Legrand P, Piras C, Vernede X, Fontecilla-Camps JC | title = Crystallization and 2.2 A resolution structure of R-phycoerythrin from Gracilaria chilensis: a case of perfect hemihedral twinning | journal = Acta Crystallographica D | volume = 57 | issue = Pt 1 | pages = 52–60 | date = January 2001 | pmid = 11134927 | doi = 10.1107/S0907444900015274 | url = http://scripts.iucr.org/cgi-bin/paper?S0907444900015274 | id = PDB ID: 1EYX }}
3. ^Image created with RasTop (Molecular Visualization Software).
4. ^{{Cite journal |url=http://www.rcsb.org/pdb/explore/explore.do?structureId=3V57 |title=Crystal Structure of the B-phycoerythrin from the red algae Porphyridium cruentum at pH8 |author=Camara-Artigas, A. |date=2011-12-16 |publisher=RCSB Protein Data Bank (PDB) |id=PDB ID: 3V57 |doi=10.2210/pdb3v57/pdb |access-date=12 October 2012}}
5. ^{{cite journal | vauthors = Camara-Artigas A, Bacarizo J, Andujar-Sanchez M, Ortiz-Salmeron E, Mesa-Valle C, Cuadri C, Martin-Garcia JM, Martinez-Rodriguez S, Mazzuca-Sobczuk T, Ibañez MJ, Allen JP | title = pH-dependent structural conformations of B-phycoerythrin from Porphyridium cruentum | journal = The FEBS Journal | volume = 279 | issue = 19 | pages = 3680–3691 | date = October 2012 | pmid = 22863205 | doi = 10.1111/j.1742-4658.2012.08730.x | id = PDB ID: 3V57 }}
6. ^MicroPlate Detection comparison between SureLight®P-3L, other fluorophores and enzymatic detection Columbia Biosciences, 2010
7. ^Cyanobacterial stabilized phycobilisomes as fluorochromes for extracellular antigen detection by flow cytometry Telford - J. Immun. Methods, 2001

4 : Photosynthetic pigments|Cyanobacteria proteins|Algae|Bacterial proteins
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