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bd oxidase; Geobacillus thermodenitrificans

1 Introduction
2 Structure

Introduction

bd oxidase is an integral membrane protein that catalyzes the reduction of O₂ -> 2H₂O using quinol as the reducing substrate. ^[1] The reaction is electrogenic but is not coupled to a proton pump. Instead, bd oxidase uses internal water molecules to provide the protons needed for the reduction reaction. ^[2] It plays a key role in protecting the organism from high oxidative stress (ie. preventing free radicals in intracellular space in prokaryotes, more specifically gram-negative heterotrophs). ^[3] There are two main types of respiratory cytochrome oxidases: the heme/copper oxidases, and the heme-only cytochrome bd quinol oxidase, which is what bd oxidase falls under. ^[4] Heme-only cytochrome bd quinol oxidases are associated with microaerobic dioxygen respiration, and they have a high affinity for oxygen.

Structure

The contains that are arranged in a nearly oval shape (Fig 1.) ^[5] The protein contains two structurally similar subunits, , and , each containing nine helices, and one smaller subunit, , with one transmembrane helix. The subunits are interacting using hydrophobic residues and symmetry at the interfaces. The CydX subunit, whose function is not currently known, is positioned in the same way as CydS, which is found in E. coli bd oxidase. Due to its similar structure and position, it has been hypothesized to potentially stabilize during potential structural rearrangements of the Q loop upon binding and oxidation of quinol ^[6]. The is a hydrophilic region above Cyd A. The lack of hydrogen bonding in this hydrophobic protein allows the protein to be flexible and go through a large conformational change for reduction of dioxygen.

Active Site

Figure 1. Heme B558 (pink; left), Heme B595 (pink; right), and Heme D (green)

The active site for Bd Oxidase in Geobacillus thermodenitrificans is located in subunit Cyd A. The site consists of three iron hemes: Heme B558, Heme B595, and Heme D that are held together in a rigid triangular due to van der waals interactions. The length between each heme's central iron is relatively constant which serves to shuttle protons and electrons from one heme to another efficiently (Fig. 1). It is suggested that Heme B558 acts as an electron acceptor to the extracellular side and Heme B559 acts as a proton acceptor on the intracellular side. It is then proposed that both heme B558 and B595 shuttle their respective ions directly to Heme D based on this being the shortest pathway (reference). Heme D is then suggested to be the oxygen binding site due to proximity and orientation to the exterior surface of the protein.

Potential Oxygen Entry Site

Heme D is the hypothesized spot for the to enter the protein . Heme D (seen in green) is directly connected to the protein surface on CydA and contains a solvent accessible substrate channel. This channel and accessibility allows for oxygen to easily bind to Heme D and eventually be reduced to 2H₂O.

Electron Source

An electron source is needed in order for the redox reaction of O₂ to occur. Bd oxidase uses the quinol molecule ubiquinone as an electron donor. The chemical structure of ubiquinone is shown in Fig. 3.

Figure 3. Chemical structure of ubiquinone.

As shown in the overall , the is on the extracellular surface and provides a binding site for ubiquinone. As mentioned in the Active Site section, Heme is closest in proximity to the Q loop and thus is the suggested electron acceptor.

Potential Proton Pathways

Figure 4. Two potential sources of protons: CydA and CydB pathway.

Because there is no proton pump present, the most likely proton transfer mechanism is facilitated by intracellular water molecules.

One potential proton pathway is formed from the four-helix bundle (a1-4) of CydA. It is called the . The location of Glu108 in our structure, together with previous mutagenesis experiments supports the proposal that this glutamate residue is a redox state-dependent mediator of proton transfer to a charge compensation site. ^[7] With the CydA pathway leading to Glu101, this residue could be the protonatable group used for charge compensation upon heme b595 reduction. It is still unknown whether protons entering the CydA pathway can be transferred from Glu101 to Glu378, to allow the spread of the negative charge of a second electron used to reduce the two high-spin hemes. Proto- nation of Glu378 could alternatively also be accomplished by a proton accessing from the extracellular side. More research needs to be done to determine whether the CydA pathway is solely providing protons for charge compensation or whether Glu108 can be a branching point that is able to pass protons via the heme b595 propionates to the oxygen-binding site.

Another potential entry site is related to the a1-4 four-helix bundle of CydB. Therefore, this is called the . In this pathway, Asp25 is thought to be the equivalent of the Glu108 in the CydA pathway ^[8]. The other residues help facilitate the movement of the proton very similarly to the CydA pathway. There is less known about the CydB pathway, and therefore, the CydA pathway is the most accepted source of protons.

Structure Similarity to Bd Oxidase found in Ecoli

The structure of Bd Oxidase for Geobacillus thermodenitrificans is highly similar to the structure of Bd Oxidase for Ecoli with the only noticeable difference being the length of the Q-loop. The similarity and differences between the two proteins can be seen in the alignment of their main structures (Fig.5).

Figure 4. Alignment of bd oxidase for the organisms Geobacillus thermodenitrificans (blue) and Ecoli (purple).

Figure 6. Heme arrangements for the organisms Geobacillus thermodenitrificans and Ecoli. Heme D shown in green; Heme B595 and Heme B558 shown in pink

Although only having one noticeable difference in structure, this difference causes the two proteins to have different active sites. In particular, the hemes of bd oxidase in Ecoli are arranged differently than the hemes in Geobacillus thermodenitrificans. The main reason for this change in heme arrangement is because of the oxygen-binding site being blocked by the Q-loop in Ecoli, thus causing oxygen to have to bind at a different binding site on the protein. The difference in the arrangement of hemes is shown in Fig. 5.

References

↑ Giuffre A, Borisov VB, Arese M, Sarti P, Forte E. Cytochrome bd oxidase and bacterial tolerance to oxidative and nitrosative stress. Biochim Biophys Acta. 2014 Jul;1837(7):1178-87. doi:, 10.1016/j.bbabio.2014.01.016. Epub 2014 Jan 31. PMID:24486503 doi:http://dx.doi.org/10.1016/j.bbabio.2014.01.016
↑ Safarian S, Hahn A, Mills DJ, Radloff M, Eisinger ML, Nikolaev A, Meier-Credo J, Melin F, Miyoshi H, Gennis RB, Sakamoto J, Langer JD, Hellwig P, Kuhlbrandt W, Michel H. Active site rearrangement and structural divergence in prokaryotic respiratory oxidases. Science. 2019 Oct 4;366(6461):100-104. doi: 10.1126/science.aay0967. PMID:31604309 doi:http://dx.doi.org/10.1126/science.aay0967
↑ Junemann S. Cytochrome bd terminal oxidase. Biochim Biophys Acta. 1997 Aug 22;1321(2):107-27. doi:, 10.1016/s0005-2728(97)00046-7. PMID:9332500 doi:http://dx.doi.org/10.1016/s0005-2728(97)00046-7
↑ Das A, Silaghi-Dumitrescu R, Ljungdahl LG, Kurtz DM Jr. Cytochrome bd oxidase, oxidative stress, and dioxygen tolerance of the strictly anaerobic bacterium Moorella thermoacetica. J Bacteriol. 2005 Mar;187(6):2020-9. doi: 10.1128/JB.187.6.2020-2029.2005. PMID:15743950 doi:http://dx.doi.org/10.1128/JB.187.6.2020-2029.2005
↑ Safarian S, Rajendran C, Muller H, Preu J, Langer JD, Ovchinnikov S, Hirose T, Kusumoto T, Sakamoto J, Michel H. Structure of a bd oxidase indicates similar mechanisms for membrane-integrated oxygen reductases. Science. 2016 Apr 29;352(6285):583-6. doi: 10.1126/science.aaf2477. PMID:27126043 doi:http://dx.doi.org/10.1126/science.aaf2477
↑ Safarian S, Rajendran C, Muller H, Preu J, Langer JD, Ovchinnikov S, Hirose T, Kusumoto T, Sakamoto J, Michel H. Structure of a bd oxidase indicates similar mechanisms for membrane-integrated oxygen reductases. Science. 2016 Apr 29;352(6285):583-6. doi: 10.1126/science.aaf2477. PMID:27126043 doi:http://dx.doi.org/10.1126/science.aaf2477
↑ Safarian S, Rajendran C, Muller H, Preu J, Langer JD, Ovchinnikov S, Hirose T, Kusumoto T, Sakamoto J, Michel H. Structure of a bd oxidase indicates similar mechanisms for membrane-integrated oxygen reductases. Science. 2016 Apr 29;352(6285):583-6. doi: 10.1126/science.aaf2477. PMID:27126043 doi:http://dx.doi.org/10.1126/science.aaf2477
↑ Safarian S, Rajendran C, Muller H, Preu J, Langer JD, Ovchinnikov S, Hirose T, Kusumoto T, Sakamoto J, Michel H. Structure of a bd oxidase indicates similar mechanisms for membrane-integrated oxygen reductases. Science. 2016 Apr 29;352(6285):583-6. doi: 10.1126/science.aaf2477. PMID:27126043 doi:http://dx.doi.org/10.1126/science.aaf2477

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@@ Line 27: / Line 27: @@
 ==Potential Proton Pathways==
-[[Image:Screen_Shot_2020-04-06_at_12.46.26_PM.png|250 px|right|thumb|Figure 6. Two potential sources of protons: CydA and CydB pathway.]]
+[[Image:Screen_Shot_2020-04-06_at_12.46.26_PM.png|250 px|right|thumb|Figure 4. Two potential sources of protons: CydA and CydB pathway.]]
 Because there is no proton pump present, the most likely proton transfer mechanism is facilitated by intracellular water molecules.
@@ Line 35: / Line 35: @@
 == Structure Similarity to Bd Oxidase found in ''Ecoli'' ==
-The structure of Bd Oxidase for ''Geobacillus thermodenitrificans'' is highly similar to the structure of Bd Oxidase for ''Ecoli'' with the only noticeable difference being the length of the Q-loop. The similarity and differences between the two proteins can be seen in the alignment of their main structures (Fig.5). [[Image:Aligmentbdoidase.jpg|200 px|right|thumb|Figure 4. Alignment of bd oxidase for the organisms ''Geobacillus thermodenitrificans'' (blue) and ''Ecoli'' (purple).]] [[Image:Heme alignment.png|200 px|left|thumb|Figure 5. Heme arrangements for the organisms ''Geobacillus thermodenitrificans'' and ''Ecoli''. Heme D shown in green; Heme B595 and Heme B558 shown in pink]] Although only having one noticeable difference in structure, this difference causes the two proteins to have different active sites. In particular, the hemes of bd oxidase in ''Ecoli'' are arranged differently than the hemes in ''Geobacillus thermodenitrificans''. The main reason for this change in heme arrangement is because of the oxygen-binding site being blocked by the Q-loop in ''Ecoli'', thus causing oxygen to have to bind at a different binding site on the protein. The difference in the arrangement of hemes is shown in Fig. 5.
+The structure of Bd Oxidase for ''Geobacillus thermodenitrificans'' is highly similar to the structure of Bd Oxidase for ''Ecoli'' with the only noticeable difference being the length of the Q-loop. The similarity and differences between the two proteins can be seen in the alignment of their main structures (Fig.5). [[Image:Aligmentbdoidase.jpg|200 px|right|thumb|Figure 4. Alignment of bd oxidase for the organisms ''Geobacillus thermodenitrificans'' (blue) and ''Ecoli'' (purple).]] [[Image:Heme alignment.png|200 px|left|thumb|Figure 6. Heme arrangements for the organisms ''Geobacillus thermodenitrificans'' and ''Ecoli''. Heme D shown in green; Heme B595 and Heme B558 shown in pink]] Although only having one noticeable difference in structure, this difference causes the two proteins to have different active sites. In particular, the hemes of bd oxidase in ''Ecoli'' are arranged differently than the hemes in ''Geobacillus thermodenitrificans''. The main reason for this change in heme arrangement is because of the oxygen-binding site being blocked by the Q-loop in ''Ecoli'', thus causing oxygen to have to bind at a different binding site on the protein. The difference in the arrangement of hemes is shown in Fig. 5.

Sandbox Reserved 1600

From Proteopedia

Revision as of 21:36, 6 April 2020

bd oxidase; Geobacillus thermodenitrificans

Contents

Introduction

Structure

Active Site

Potential Oxygen Entry Site

Electron Source

Potential Proton Pathways

Structure Similarity to Bd Oxidase found in Ecoli

References

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