We used Pfam [16] hidden Markov models for 53 DNA-binding domains (see Materials and methods) to search all proteins in SWISS-PROT/TrEMBL [17] and SwissPfam protein databases. The 9,261 proteins identified by our search are presumed members of DNA-binding protein families, and most are expected to be transcription factors. These proteins were then scored for the presence of one or more transmembrane segments using prediction programs PHDhtm [l8], TMHMM [19], HMMTOP [20] and PSORTII [21]. Only those proteins containing membrane-spanning helices predicted by at least three of the four programs were deemed significant in our analysis. By these stringent criteria, 76 proteins from 20 organisms and one virus were identified as putative TMTFs (Figure 1).

Our analysis predicted a surprisingly large and diverse set of membrane-tethered DNA-binding proteins. Seventeen of the 53 DNA-binding domains chosen for this analysis were represented in the final set of TMTFs. Of these, the most abundant is the zf-C4 (zinc-finger type C4) nuclear hormone receptor DNA-binding domain, found in 14 proteins in Caenorhabditis elegans and avian erythroblastosis virus. TMTFs in Arabidopsis were the most diverse, and were associated with eight different DNA-binding domains. All but two proteins have DNA-binding domains that could be separated from the rest of the protein by a single hypothetical cleavage event, if singly predicted transmembrane segments are discounted (Figure 1). DNA-binding domains were also frequently juxtaposed to bipartite nuclear localization signals, suggesting that transmembrane and DNA-binding domains in TMTFs are modular. Thus, the overall topology of these proteins is consistent with other known TMTFs. C. elegans has an impressive 25 predicted TMTFs, suggesting that RIP may be particularly important in the regulation of transcriptional responses in the worm. Interestingly, 56 of the 76 identified proteins lack any experimental annotation.

We deliberately used a stringent method to increase the likelihood of identifying only bona fide TMTFs and, as expected, most experimentally known TMTFs were detected by our analysis, including CadC [5], Lzip [7], ToxR [6] and all SWISS-PROT/TrEMBL orthologs of SREBP-l and SREBP-2. Also found were several well-characterized proteins whose predicted membrane insertion had not been recognized. For example, the human doublesex-related protein DMRT2, Drosophila B-H2 (BarH2) protein, C. elegans UNC-86, and mouse OASIS protein are predicted TMTFs. Two known TMTFs, ATF6 and SPT23, did not satisfy our minimum criteria. The transmembrane helix of ATF6 was predicted by only two programs: PSORT and HMMTOP. The immunoglobulin DNA-binding domain (TIG) of SPT23 is found in both cell-surface proteins as well as transcription factors and was therefore excluded from the set of DNA-binding domains. These results indicate that reducing the stringency of our prediction method will expand the number of predicted TMTFs.

In some cases we found data in the literature to support our computational predictions. For example, cell-fractionation studies using antibodies directed at the carboxyl terminus of the chaperonin MTJ1 showed that the full-length (62 kDa) protein exists in microsomes, whereas a smaller 42 kDa form of the protein is found in the nucleus [15]. The 42 kDa species was hypothesized to represent a product of internal translation. Because MTJ1 contains putative Myb DNA-binding domains within the carboxy-terminal half of the protein, we re-examined the subcellular localization of carboxy-terminal-tagged MTJ1 in COS-7 cells (Figure 2a). Our results show clearly that full-length MTJ1 is normally associated with the endoplasmic reticulum. In contrast, a truncated form MTJ1Δ (approximately 40 kDa in size) lacking the transmembrane segment accumulates in the nucleus. Therefore, we propose that the 42 kDa nuclear form of MTJ1 observed in cells arises by cleavage of MTJ1 from the membrane, rather than from aberrant translation of the mRNA.

DMRT2, a human homolog of C. elegans mab-3, was identified in our analysis as having a carboxy-terminal transmembrane segment (Figure 1). mab-3 encodes a transcription factor known for its role in sex determination in worms [22]. DMRT2 has gained recent attention as a candidate gene for sex-reversal phenotypes in humans [23]. To verify our prediction that DMRT2 is a membrane-tethered transcription factor, we examined the subcellular localization of full-length and truncated forms of DMRT2 in COS-7 cells (Figure 2b). Full-length DMRT2 is localized primarily, but not exclusively, to vesicles outside the nucleus. A carboxy-terminal truncation containing the DNA-binding domain is, however, concentrated almost entirely in the nucleus. These results are consistent with the idea that DMRT2 is cleaved from the membrane to produce a nuclear fragment. Interestingly, transformer protein TRA-2A, an indirect activator of MAB-3, has been identified recently as a membrane-tethered nuclear protein [24,25]. Thus, RIP maybe a conserved mechanism common to sex determination in humans and worms.

Pfam [16] hidden Markov models for 53 DNA-binding domains (see DNA-binding domains below) were used to search proteins in SWISS-PROT/TrEMBL (October 2000 release; 388,909 proteins) with p-value < 0.0019 (0.01/53). SwissPfam proteins identified as having any of the 53 domains were also included in our analysis. The resulting 9,261 proteins were then analyzed for the presence of transmembrane helices. Default parameters were used for HMMTOP [20], PHDhtm [l8], and TMHMM (version 2 [19]). A higher stringency (-5.0) than default was used for PSORT II (ALOM2 [21]). Transmembrane segments predicted by individual programs were considered overlapping if ten or more amino acids were shared by each segment. Proteins containing transmembrane helices predicted by at least three of the four programs were included in the final set. Bipartite nuclear localization signals were identified using PSORT II. Three predicted TMTFs were discounted as false-positives on the basis of partial or complete overlap of transmembrane helices with other Pfam domains (O01612, O23045 and Q13771).

The following Pfam models for DNA-binding domains were used (abbreviated as in Pfam): 7 kDa DNA-binding; AP2-domain; ARID; ASNC trans reg; AT hook; Arg represser; B3; BAH; BRO; Bac DNA-binding; basic; bZIP; CBFB NFYA; CSD; CUT; copper-fist; DM-domain; E2F TDP; fork head; GATA; HALZ; HLH; homeobox; HSF DNA-binding; HTH 3; HTH 4; HTH 5; IRF; LexA DNA-binding; MBD; MetJ; Myb DNA-binding; MutS N; Myc-LZ; PHD; RFX DNA-binding; RHD; Runt; SAP; sigma70; SRF-TF; STAT; sigma54 factors; sigma70 ECF; T-box; TBP; yeast DNA-binding; Trans reg C; zf (zinc finger)-C2H2; zf-C2HC; zf-C4; zf-NF-X1; Zn-clus.

Full-length DMRT2 and MTJ1Δ were generated by PCR using Pfu polymerase (Stratagene) and cloned directionally into BamHI/XbaI sites of pCDNA3 (Invitrogen). Truncated MTJ1, in which an ATG (methionine) was added immediately before amino acid 171 (Q61712), was amplified from expressed sequence tag (EST) AI790297 (Incyte Genomics) and a Myc tag was added at the carboxyl terminus. MTJ1Δ -forward primer: 5'-CGCGGATCCGCGATGGAAAAGCAACTGGATGAACTG-3'. MTJ1Δ -reverse primer: 5'-GCTCTAGAGCTACAGGTCCTCCTCCGAGATGAGTTTCTGTTCCATGCTTTTAGCCTGCTTTTTCTT-3'. The ATG in bold indicates the translation start site of truncated MTJ1. Full-length MTJ1 was prepared by digesting clone AI790297 with XhoI, blunting ends, then digesting with EcoRI. This fragment was then cloned into pcDNA3-MTJ1Δ, which was digested with BamHI, blunt-ended, and digested with EcoRI. Full-length and truncated DMRT2 (at amino acid 180; Q9Y5R5) were amplified from EST AI985131 (Incyte), and a Myc tag was added at the amino terminus. DMRT2-forward primer: 5'-CGCGGATCCGCGATGGAACAGAAACTCATCTCGGAGGAGGACCTGATGGCCGACCCGCAGG-3'. DMRT2-reverse primer: 5'-GCTCTAGAGCTAAAGATGGTTCATTATGTAC-3'. DMRT2Δ -reverse primer: 5'-GCTCTAGAGTCAGGCTCTGACTTGCCTCTG-3'.

Standard DEAE transfections [26] of plasmids were done in COS-7 cells (ATCC) and grown in 10% FBS/DMEM. Cells were fixed 72 h post-transfection in 3% PFA in PBS and Myc tags were detected with mouse anti-Myc antibodies (NeoMarkers, Fremont, CA) and Texas-Red-X goat anti-mouse antibodies (Molecular Probes, Eugene, OR) using standard procedures. Nuclei were counterstained with Hoechst 33258. Photomicrographs were taken on a Zeiss Axiophot.