Amino Acids of Conserved Kinase Motifs of Cytomegalovirus Protein UL97 Are Essential for Autophosphorylation

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Journal of Virology, October 1999, p. 8898-8901, Vol. 73, No. 10
0022-538X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Amino Acids of Conserved Kinase Motifs of Cytomegalovirus Protein UL97 Are Essential for Autophosphorylation

Detlef Michel, Silke Kramer, Simone Höhn, Peter Schaarschmidt, Kirsten Wunderlich, and Thomas Mertens^*

Abteilung Virologie, Institut für Mikrobiologie und Immunologie, Universitätsklinikum Ulm, 89081 Ulm, Germany

Received 3 May 1999/Accepted 15 July 1999

	ABSTRACT

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Thirteen point mutations targeting predicted domains conserved in homologous protein kinases were introduced into the UL97coding region of the human cytomegalovirus. All mutagenized proteinswere expressed in cells infected with recombinant vaccinia viruses(rVV). Several mutations drastically reduced ganciclovir (GCV)phosphorylation. Mutations at amino acids G340, A442, L446, andF523 resulted in a complete loss of pUL97 phosphorylation, whichwas strictly associated with a loss of GCV phosphorylation. Ourresults confirm that in rVV-infected cells pUL97 phosphorylationis due to autophosphorylation and show that several amino acidsconserved within domains of protein kinases are essential forthis pUL97 phosphorylation. GCV phosphorylation is dependent onpUL97phosphorylation.

	TEXT

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It has been shown that open reading frame (ORF) UL97 of human cytomegalovirus (HCMV) encodes a protein that has homologieswith protein kinases (PK) but that also directs the essentialphosphorylation of ganciclovir (GCV) and other antiviral nucleosideanalogs to their monophosphates (2, 11, 19, 24). TheUL97 protein (pUL97) is detectable in the nuclei of infected andtransfected cells but is not localized in the nucleoli (15).Multiple clustered mutations in the coding region of UL97 havebeen described to induce phenotypical resistance to GCV in HCMVstrains (1, 3, 7, 12, 19, 23). Until now, no clinicalHCMV strains carrying extensive deletions or lacking pUL97 havebeenisolated.

Although investigated by different groups, the biological relevance of UL97 is still unknown. Very recently it has been publishedthat a recombinant HCMV with a large deletion in UL97 has a severereplication deficiency (16a). pUL97 is present in the virus particlesand is able to partially substitute in function for the herpessimplex virus UL13 protein (16, 21, 22). Evidence obtainedfrom recombinant vaccinia viruses (rVV) indicated that pUL97 isnot a nucleoside kinase (14). Furthermore, it was shown that,after expression in the baculovirus system, the protein autophosphorylatesat serines and threonines (8). By investigating pUL97 derivativescarrying larger deletions in the vaccinia virus system, we couldshow that the N terminus contains a nuclear localization signaland that a central domain (amino acids [aa] 305 to 365) is essentialfor pUL97 phosphorylation as well as for GCV phosphorylation (15).Only one artificial amino acid exchange has been published sofar, proving the importance of an invariant lysine at position355 for autophosphorylation (8).

In PK from different species, several domains, I to XI, have been defined by sequence alignments (5, 6). Very recentlythe crystal structure of the type I transforming growth factor $beta$ receptor with an autophosphorylating serine/threonine kinaseactivity has also been reported to contain these regions (9).In pUL97, homologous sequences have been found for the PK domains(Fig. 1). However, an additional putative functional domain whichis not detectable in PK seems to be located between domains VIIand VIII. Since no other natural substrate has been identifiedso far, even today the assumption that pUL97 is a PK is basedmainly on the above-mentioned partial sequence homologies andon the autophosphorylating capacity of the protein.

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FIG. 1. Alignment of some conserved motifs in different UL97 homologues. The numbers indicate amino acid positions of the UL97 protein sequence. Published mutations conferring GCV phenotypic resistance on HCMV strains are indicated by boldface, underlined, italic letters. Domain, conserved domains in PK as defined by Hanks et al. (5, 6); S/T-PK, amino acids conserved in serine/threonine PK; Herp, amino acids that are conserved in the UL97 homologues of herpes simplex virus, human herpesvirus 6, varicella-zoster virus, and Epstein-Barr virus according to the work of Chee et al. (2); RhCMV, rhesus cytomegalovirus; MCMV, murine cytomegalovirus; GCMV, guinea pig cytomegalovirus (4, 20); Cons, amino acids that are conserved among the cytomegalovirus proteins; MUTA, mutations introduced by site-directed mutagenesis.

Site-directed mutagenesis in the UL97 ORF. Very few amino acids conserved in PK have been proven experimentally to be indispensable for the functions of these proteins,an example being the GXGXXG motif involved in nucleotide bindingin domain I or the invariant lysine in domain II (2, 6).In addition, by sequence alignments conserved amino acids or evensequence motifs implicating functional relevance and allowingfor the definition of different conserved motifs have been detected.In order to get further evidence for the PK nature of pUL97, wewanted to experimentally prove the existence of assumed functionalregions of the viral protein that are obviously involved in phosphorylation.Therefore, site-directed mutagenesis was performed at specificamino acids in different domains which are conserved among thepUL97 homologues of different cytomegaloviruses, human herpesviruses,and nonviral serine/threonine kinases, including the PK regionof the transforming growth factor $beta$ receptor (9). Other mutationswere introduced in the vicinities of putative functional aminoacids in order to estimate the extension of the presumed domains(Fig. 1). None of the mutations have been found in phenotypicallyresistant HCMV. We also introduced a stop codon at aa Y617 totruncate the protein beyond this position. Therefore, from plasmidp214 containing the entire pUL97 coding region (14, 17) aBamHI/EcoRI fragment, aa 20 to 707, was extracted. After thisfragment was introduced into plasmid pALTER (Promega), site-directedmutagenesis was performed by using the following oligonucleotides:335Y>D, 5'-C ATG AGC GAC GAG AGC GAC CGC CTG-3'; 340G>V,5'-GGC CAG GTC TCC TTC GGC-3'; 354V>L, 5'-C TAT CGC GTGCTC AAG GTG-3'; 359K>Q, 5'-G GCG CGT CAG CAC AGCGAG ACG-3'; 380E>V, 5'-GCT GGC GTG CAA CAG CAG C-3'; 442A>V,5'-C ACG TTG GCC GAC GTT ATC AAA TT-3'; 446L>R, 5'-TTTCGC AAT CAC CAG TGT CG-3'; 523F>C, 5'-CAC CCT GCT TGCCGA CCC ATG CCG C-3'; 526M>I, 5'-GCT TTC CGA CCC ATC CCGCTG CAG AAG-3'; 574D>A, 5'-CGG CGC GGT CTG GCC GAG GTGCGC-3'; 579G>A, 5'-G CGC ATG GCC ACG GAG G-3'; 583L>F,5'-G GAG GCG TTT CTC TTT AAG-3'; and 617Y>Stop, 5'-A ATGAGC TAA GGC GCC TGT CTC CTG-3' (where underlining indicatesthe presumed functional amino acid and boldface indicates themutationintroduced).

Expression of the pUL97 derivatives after infection with rVV. The mutagenized UL97 coding regions were introduced into vaccinia viruses in order to test functional properties, i.e., nuclearlocalization, GCV phosphorylation, and pUL97 phosphorylation.The expression of all mutagenized UL97 derivatives was confirmedby Western blot analysis (10) (Fig. 2A). None of the mutationsdisturbed the intracellular localization of the UL97 proteins,which were all found in the nuclei of infected cells (data notshown). However, the migrations and shapes of the different pUL97signals in the Western blot were dependent on the ability to phosphorylatepUL97 itself (see Fig. 2B and below). Loss of this function resultedin a sharp band at 80 or 70 kDa for rVV617, whereas autophosphorylationcaused an apparently more intensive signal. However, these signalswere due mainly to several additional, slower-migrating bands,resulting in a smear between 80 and approximately 100 kDa. Nosignals were observed in cell extracts harvested after mock infectionor after infection with the wild-type vaccinia virus strain Copenhagencarrying the thymidine kinase of vaccinia virus.

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FIG. 2. Expression and phosphorylation of newly mutagenized UL97 proteins in cells infected with rVV. Lanes labeled 335 to 617 indicate rVV carrying different point mutations in the UL97 ORF introduced by site-directed mutagenesis; cop, cells infected with the vaccinia virus strain Copenhagen (without the UL97 ORF). CV1 cells were infected at an MOI of 5 with the indicated rVV and were harvested 17 to 20 h postinfection for preparation of nuclear extracts. The extracts were used in parallel for both Western blot analyses and PK assays. (A) For Western blotting nuclear matrix extracts were separated by sodium dodecyl sulfate-12% polyacrylamide gel electrophoresis. Here pUL97 was visualized by chemiluminiscence with the pUL97 antiserum. (B) For determination of pUL97 phosphorylation, nuclear matrix fractions were tested for PK activity. Proteins were resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and visualized by autoradiography.

GCV phosphorylation and phosphorylation of pUL97 in cells infected with rVV. Two advantages of the pUL97 vaccinia virus system are the possibilities of quite easily generating recombinants (13) andof investigating mutated UL97 proteins that might cause a nongrowingor slow-growing HCMV phenotype. Since purification of the foreignprotein, biochemical quantification, and in vitro enzymology havenot been possible so far, we have performed extensive experimentsto correlate the multiplicities of the infecting vaccinia viruseswith pUL97 expression, quantitative GCV phosphorylation, and pUL97phosphorylation (18). Quantitative determination of GCV phosphorylationwith a standard deviation of 20% was possible when a multiplicityof infection (MOI) between 10 and 40 was used (18). Hence, forall GCV phosphorylation experiments in this study 143B (tk) cells were infected with vaccinia virus recombinants at an MOIof 20. High-pressure liquid chromatography analysis was performedas described previously (14, 24). For fractionation of nucleiand cytoplasms, CV1 cells were infected with rVV at an MOI of5 and harvested 20 h postinfection as described previously (14,24). Phosphorylation of pUL97 was determined according to themethod of He et al. (8). The phosphorylating capacities ofthe different UL97 mutants in the rVV-infected cells are summarizedin Fig. 3, whereas the data showing the phosphorylation of pUL97itself are shown in Fig. 2B. Two point mutations at D574 and G579,amino acids conserved in UL97 homologues of other herpesviruses,as well as the nearby mutation at L583 (all domain IX [Fig. 1])in the N-terminal part of the region, where most of the naturalmutations that confer GCV resistance are clustered (aa 591, 592,594, 595, 596, 598, 603, and 607) (1, 3, 7, 12, 18,19, 23), did not interfere with GCV or pUL97 phosphorylation.However, the stop codon at the tyrosine at position 617 causeda complete loss of GCV phosphorylation and of pUL97 phosphorylationas well, suggesting that the region beyond the stop codon is alsoinvolved in protein function.

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FIG. 3. GCV phosphorylation in rVV-infected 143B (thymidine kinase-deficient) cells. The numbers 335 to 617 indicate the different rVV; cop, vaccinia virus strain Copenhagen. The bars represent mean values and standard errors of the results of 6 to 10 independent experiments. The Roman numerals denote conserved domains in PK (5). Point mutations which were found in phenotypically resistant HCMV at positions 460, 520, and 594 have been previously described (14) and are indicated by asterisks. The invariant lysine (K) at position 355 reported by He et al. (8) is indicated.

The substitution of the second glycine residue at position 340 of the highly conserved GXGXXG motif which is part of domainI of PK and involved in nucleotide binding resulted in the completeloss of GCV phosphorylation and pUL97 phosphorylation. Interestingly,the alteration of the Y amino acid at position 335, located only5 aa upstream of this crucial position, only slightly influencedGCV phosphorylation and did not inhibit pUL97 phosphorylation.The substitution of the lysine at position 359, which we had suspectedto be the invariant lysine of PK (15), did not lead to the expectedloss of GCV or pUL97 phosphorylation, although a decline of approximately50% was measured in GCV phosphorylating activity. The mutationof the adjacent V354 did not influence either phosphorylatingactivity. This result is in accordance with the assumption thatit is in fact the lysine located at a typical distance of 14 aafrom the GXGXXG domain that is essential for phosphatebinding.

The glutamic acid of PK in domain III can be detected only in some of the viral pUL97 homologues. However, it is found inthe protein derived from human herpesvirus 6 and in pUL97, whereit is supposed to be located at position 380. The substitutionof this amino acid caused only a small decrease in GCV phosphorylationand no alteration in pUL97phosphorylation.

Contrary to this small decrease, dramatic effects were observed with the substitutions A442V, L446R, and F523C. The firstand second were located in domain VIa, and the last was locatedin the putative specific domain unique for UL97 homologues ofherpesviruses. All three point mutations conferred a completeloss of GCV phosphorylation down to levels observed in mock-infectedcells and also a loss of pUL97 phosphorylation. It should be mentionedthat both of the two mutations (M460V and H520O) from naturallyresistant HCMV strains found in this regions drastically reducedGCV phosphorylation but not pUL97 phosphorylation (15). Untilnow only reductions in GCV phosphorylation have been observedfor GCV-resistant clinical isolates. It is even more significantthat all point mutations or small deletions found in pUL97s ofHCMV isolates gave rise to proteins which were still able to autophosphorylatewhen they were investigated with our vaccinia virus system (14,15, 18). Together with the known fact that phosphorylationis a widespread mechanism of activation or inactivation in biologicalsystems, our results strengthen the view that autophosphorylationof the protein may well be associated with its natural, biologicalfunction. Additionally, we could demonstrate for the first timethat autophosphorylation seems to be a prerequisite for GCV phosphorylation,since mutations abrogating autophosphorylation concomitantly ledto a complete loss of GCVphosphorylation.

Phosphorylation of pUL97 expressed by rVV is also due to autophosphorylation. In conclusion, rVV-expressed pUL97 is biologically active as determined by GCV phosphorylation. Under the conditions used(1 M NaCl and pH 9.0), an 80-kDa protein was the major labeledspecies in the nuclear matrix fractions (Fig. 2B). These labeledproteins comigrated with pUL97 as detected by parallel Westernblot analysis performed with identical samples (Fig. 2A). However,the phosphorylated protein at 80 kDa was not observed with rVV340,rVV442, rVV446, rVV523, or rVV617, whereas in the Western blotanalysis the 80-kDa proteins were present in all samples testedexcept for rVV617, which produced a smaller band since the proteinwas C-terminally truncated. Virtually no comparable labeling at80 kDa was observed when nuclear matrix extracts of mock-infected143B (thymidine kinase-deficient) cells or 143B cells infectedwith the wild-type vaccinia virus strain Copenhagen were incubatedwith [ $gamma$ -³³P]ATP.

To further examine whether pUL97 phosphorylation in the vaccinia virus system is indeed due to autophosphorylation, proteinphosphorylation was investigated under higher-concentration saltconditions (1.5 M NaCl), with a shorter incubation time (20 min),and in the presence of heparin (50 µg/ml). pUL97 phosphorylationwas still observed under these conditions (data not shown). Finally,we performed a time kinetic analysis of pUL97 phosphorylation,which showed that after 30 s of incubation, almost 50% of theprotein was already phosphorylated and that after 10 min, thereaction reached its maximum (data not shown). In conclusion,these findings further support the presence of an intrinsic PKactivity in pUL97 as well as in the vaccinia virus system, andthe activity seems not to be derived from contaminations in thenuclearextracts.

Here, we could show that several amino acids which are conserved among serine/threonine kinases and which can also be foundin pUL97 and its homologues in herpesviruses have a functionalrelevance for pUL97. The region present in the herpesvirus proteinsbut which is not found in the S/T PK might be connected with thesubstrate and the function of the protein. We could show for thefirst time that phosphorylation of pUL97 is essential for GCVphosphorylation. The existence of amino acids indispensable forprotein function again indicate that pUL97 may be an interestingdirect target for antiviraltherapy.

	ACKNOWLEDGMENTS

The skillful technical assistance of Anke Lüske and the valuable help of Albert Zimmermann in the performance of the high-pressureliquid chromatography analyses and the kinase assays are greatlyappreciated.

P.S. is a student of the DFG-Graduiertenkolleg Biomolekulare Medizin; D.M. was supported by a grant of the BMBF (01KI9603).The work was supported in part by a grant from the European community(PL960471).

	FOOTNOTES

^* Corresponding author. Mailing address: Abteilung Virologie, Institut für Mikrobiologie und Immunologie, UniversitätsklinikumUlm, Albert-Einstein-Allee 11, 89081 Ulm, Germany. Phone: 49 7315023341. Fax: 49 731 5023337. E-mail: thomas.mertens{at}medizin.uni-ulm.de.

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1.	Baldanti, F., E. Silini, A. Sarasini, C. L. Talarico, S. C. Stanat, K. K. Biron, M. Furione, F. Bono, G. Palu, and G. Gerna. 1995. A three-nucleotide deletion in the UL97 open reading frame is responsible for the ganciclovir resistance of a human cytomegalovirus clinical isolate. J. Virol. 69:796-800[Abstract].
2.	Chee, M. S., G. L. Lawrence, and B. G. Barrell. 1989. Alpha-, beta- and gammaherpesviruses encode a putative phosphotransferase. J. Gen. Virol. 70:1151-1160[Abstract/Free Full Text].
3.	Chou, S., A. Erice, M. C. Jordan, G. M. Vercellotti, K. R. Michels, C. L. Talarico, S. C. Stanat, and K. K. Biron. 1995. Analysis of the UL97 phosphotransferase coding sequence in clinical cytomegalovirus isolates and identification of mutations conferring ganciclovir resistance. J. Infect. Dis. 171:576-583[Medline].
4.	Fox, D. S., and M. R. Schleiss. 1997. Sequence and transcriptional analysis of the guinea pig cytomegalovirus UL97 homolog. Virus Genes 15:255-264[Medline].
5.	Hanks, S., and A. M. Quinn. 1991. Protein kinase catalytic domain sequence database: identification of conserved features of primary structure and classification of family members. Methods Enzymol. 200:38-81[Medline].
6.	Hanks, S. K., A. M. Quinn, and T. Hunter. 1988. The protein kinase family: conserved features and deduced phylogeny of the catalytic domains. Science 241:42-52[Abstract/Free Full Text].
7.	Hanson, M., L. C. Preheim, S. Chou, C. L. Talarico, K. K. Biron, and A. Erice. 1995. Novel mutation in the UL97 gene of a clinical cytomegalovirus strain conferring resistance to ganciclovir. Antimicrob. Agents Chemother. 39:1204-1205[Abstract].
8.	He, Z., Y. He, Y. Kim, L. Chu, C. Ohmstede, K. K. Biron, and D. M. Coen. 1997. The human cytomegalovirus UL97 protein is a protein kinase that autophosphorylates on serines and threonines. J. Virol. 71:405-411[Abstract].
9.	Huse, M., Y.-G. Chen, J. Massagué, and J. Kuriyan. 1999. Crystal structure of the cytoplasmic domain of the type I TGF $beta$ receptor in complex with FKBP12. Cell 96:425-436[Medline].
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