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Conserved domains on  [gi|1110759458|ref|WP_071984141|]
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tyrosine-type recombinase/integrase [Borreliella bissettiae]

Protein Classification

site-specific integrase( domain architecture ID 332)

tyrosine based site-specific recombinase (integrase) is involved in cleavage of a single strand of a DNA duplex by nucleophilic attack of a conserved tyrosine to give a 3' phosphotyrosyl protein-DNA adduct

CATH:  1.10.443.10
Gene Ontology:  GO:0015074|GO:0003677|GO:0006310
PubMed:  10577069|10047575|9278480
SCOP:  4002347

Graphical summary

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List of domain hits

 Name Accession Description Interval E-value
DNA_BRE_C super family cl00213
DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme ...
 65-226 5.81e-05

DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme superfamily includes type IB topoisomerases and tyrosine based site-specific recombinases (integrases) that share the same fold in their catalytic domain containing conserved active site residues. The best-studied members of this diverse superfamily include Human topoisomerase I, the bacteriophage lambda integrase, the bacteriophage P1 Cre recombinase, the yeast Flp recombinase, and the bacterial XerD/C recombinases. Their overall reaction mechanism is essentially identical and involves cleavage of a single strand of a DNA duplex by nucleophilic attack of a conserved tyrosine to give a 3' phosphotyrosyl protein-DNA adduct. In the second rejoining step, a terminal 5' hydroxyl attacks the covalent adduct to release the enzyme and generate duplex DNA. The enzymes differ in that topoisomerases cleave and then rejoin the same 5' and 3' termini, whereas a site-specific recombinase transfers a 5' hydroxyl generated by recombinase cleavage to a new 3' phosphate partner located in a different duplex region. Many DNA breaking-rejoining enzymes also have N-terminal domains, which show little sequence or structure similarity.


The actual alignment was detected with superfamily member cd00397:

Pssm-ID: 469662 [Multi-domain]  Cd Length: 167  Bit Score: 42.47  E-value: 5.81e-05
                          10        20        30        40        50        60        70        80
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458  65 IIKCVKTLKHIDPISGWFVHLLVISGCRGAELQKVKMQDISTflsktgkTLYNIKVNvAKKKFTTCSREFVITEKEFNAI 144
Cdd:cd00397     5 LLDAIDEDKKIDLRDRAILLLLLETGLRISELLALKVKDIDL-------DNGTIRVR-GKKTKGGKERTVPLPKELAEEL 76

                          90       100       110       120       130       140       150       160
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458 145 QKvHENYFKEKNLNTSRTYFFQKTKLRFKDNRISIDHIAKKFKKLLRKWGFKTnkSLHLCRNLFIFNLKSNGYNSFQIKE 224
Cdd:cd00397    77 KE-YLKERRDKRGPLLKSLYLNKLFGTKLGERLSRRTLRRIFKKAGIEAGRKI--TPHSLRHTFATNLLENGVDIKVVQK 153


                  ..
gi 1110759458 225 LM 226
Cdd:cd00397   154 LL 155
 
Name Accession Description Interval E-value
DNA_BRE_C cd00397
DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme ...
 65-226 5.81e-05

DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme superfamily includes type IB topoisomerases and tyrosine based site-specific recombinases (integrases) that share the same fold in their catalytic domain containing conserved active site residues. The best-studied members of this diverse superfamily include Human topoisomerase I, the bacteriophage lambda integrase, the bacteriophage P1 Cre recombinase, the yeast Flp recombinase, and the bacterial XerD/C recombinases. Their overall reaction mechanism is essentially identical and involves cleavage of a single strand of a DNA duplex by nucleophilic attack of a conserved tyrosine to give a 3' phosphotyrosyl protein-DNA adduct. In the second rejoining step, a terminal 5' hydroxyl attacks the covalent adduct to release the enzyme and generate duplex DNA. The enzymes differ in that topoisomerases cleave and then rejoin the same 5' and 3' termini, whereas a site-specific recombinase transfers a 5' hydroxyl generated by recombinase cleavage to a new 3' phosphate partner located in a different duplex region. Many DNA breaking-rejoining enzymes also have N-terminal domains, which show little sequence or structure similarity.


Pssm-ID: 271175 [Multi-domain]  Cd Length: 167  Bit Score: 42.47  E-value: 5.81e-05
                          10        20        30        40        50        60        70        80
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458  65 IIKCVKTLKHIDPISGWFVHLLVISGCRGAELQKVKMQDISTflsktgkTLYNIKVNvAKKKFTTCSREFVITEKEFNAI 144
Cdd:cd00397     5 LLDAIDEDKKIDLRDRAILLLLLETGLRISELLALKVKDIDL-------DNGTIRVR-GKKTKGGKERTVPLPKELAEEL 76

                          90       100       110       120       130       140       150       160
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458 145 QKvHENYFKEKNLNTSRTYFFQKTKLRFKDNRISIDHIAKKFKKLLRKWGFKTnkSLHLCRNLFIFNLKSNGYNSFQIKE 224
Cdd:cd00397    77 KE-YLKERRDKRGPLLKSLYLNKLFGTKLGERLSRRTLRRIFKKAGIEAGRKI--TPHSLRHTFATNLLENGVDIKVVQK 153


                  ..
gi 1110759458 225 LM 226
Cdd:cd00397   154 LL 155
 
Name Accession Description Interval E-value
DNA_BRE_C cd00397
DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme ...
 65-226 5.81e-05

DNA breaking-rejoining enzymes, C-terminal catalytic domain; The DNA breaking-rejoining enzyme superfamily includes type IB topoisomerases and tyrosine based site-specific recombinases (integrases) that share the same fold in their catalytic domain containing conserved active site residues. The best-studied members of this diverse superfamily include Human topoisomerase I, the bacteriophage lambda integrase, the bacteriophage P1 Cre recombinase, the yeast Flp recombinase, and the bacterial XerD/C recombinases. Their overall reaction mechanism is essentially identical and involves cleavage of a single strand of a DNA duplex by nucleophilic attack of a conserved tyrosine to give a 3' phosphotyrosyl protein-DNA adduct. In the second rejoining step, a terminal 5' hydroxyl attacks the covalent adduct to release the enzyme and generate duplex DNA. The enzymes differ in that topoisomerases cleave and then rejoin the same 5' and 3' termini, whereas a site-specific recombinase transfers a 5' hydroxyl generated by recombinase cleavage to a new 3' phosphate partner located in a different duplex region. Many DNA breaking-rejoining enzymes also have N-terminal domains, which show little sequence or structure similarity.


Pssm-ID: 271175 [Multi-domain]  Cd Length: 167  Bit Score: 42.47  E-value: 5.81e-05
                          10        20        30        40        50        60        70        80
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458  65 IIKCVKTLKHIDPISGWFVHLLVISGCRGAELQKVKMQDISTflsktgkTLYNIKVNvAKKKFTTCSREFVITEKEFNAI 144
Cdd:cd00397     5 LLDAIDEDKKIDLRDRAILLLLLETGLRISELLALKVKDIDL-------DNGTIRVR-GKKTKGGKERTVPLPKELAEEL 76

                          90       100       110       120       130       140       150       160
                  ....*....|....*....|....*....|....*....|....*....|....*....|....*....|....*....|
gi 1110759458 145 QKvHENYFKEKNLNTSRTYFFQKTKLRFKDNRISIDHIAKKFKKLLRKWGFKTnkSLHLCRNLFIFNLKSNGYNSFQIKE 224
Cdd:cd00397    77 KE-YLKERRDKRGPLLKSLYLNKLFGTKLGERLSRRTLRRIFKKAGIEAGRKI--TPHSLRHTFATNLLENGVDIKVVQK 153


                  ..
gi 1110759458 225 LM 226
Cdd:cd00397   154 LL 155
 
Blast search parameters
Data Source: Precalculated data, version = cdd.v.3.21
Preset Options:Database: CDSEARCH/cdd   Low complexity filter: no  Composition Based Adjustment: yes   E-value threshold: 0.01

References:

  • Wang J et al. (2023), "The conserved domain database in 2023", Nucleic Acids Res.51(D)384-8.
  • Lu S et al. (2020), "The conserved domain database in 2020", Nucleic Acids Res.48(D)265-8.
  • Marchler-Bauer A et al. (2017), "CDD/SPARCLE: functional classification of proteins via subfamily domain architectures.", Nucleic Acids Res.45(D)200-3.
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