©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Characterization of S-AKAP84, a Novel Developmentally Regulated A Kinase Anchor Protein of Male Germ Cells (*)

(Received for publication, June 14, 1995; and in revised form, August 16, 1995)

Reigh-Yi Lin (1) Stuart B. Moss (2) Charles S. Rubin (1)

From the  (1)Department of Molecular Pharmacology, Atran Laboratories, Albert Einstein College of Medicine, Bronx, New York, 10461 and the (2)Department of Obstetrics and Gynecology, Division of Reproductive Biology, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

In mammalian spermatozoa, most of the type IIalpha isoform of cAMP-dependent protein kinase (PKAIIalpha) is anchored at the cytoplasmic surface of a specialized array of mitochondria in the flagellar cytoskeleton. This places the catalytic subunits of PKAIIalpha in proximity with potential target substrates in the cytoskeleton. The mechanism by which PKAIIalpha is anchored at the outer surface of germ cell mitochondria has not been elucidated. We now report the cloning of a cDNA that encodes a novel, germ cell A kinase anchor protein (AKAP) designated S-AKAP84. S-AKAP84 comprises 593 amino acids and contains a centrally located domain that avidly binds regulatory subunits (RIIalpha and RIIbeta) of PKAIIalpha and PKAIIbeta. The 3.2-kilobase S-AKAP84 mRNA and the cognate S-AKAP84 RII binding protein are expressed principally in the male germ cell lineage. Expression of S-AKAP84 is tightly regulated during development. The protein accumulates as spermatids undergo nuclear condensation and tail elongation. The timing of S-AKAP84 expression is correlated with the de novo accumulation of RIIalpha and RIIbeta subunits and the migration of mitochondria from the cytoplasm (round spermatids) to the cytoskeleton (midpiece in elongating spermatids). Residues 1-30 at the NH(2) terminus of S-AKAP84 constitute a putative signal/anchor sequence that may target the protein to the outer mitochondrial membrane. Immunofluorescence analysis demonstrated that S-AKAP84 is co-localized with mitochondria in the flagellum.


INTRODUCTION

Multiple isoforms of cAMP-dependent protein kinase (PKA) (^1)are expressed during mammalian spermatogenesis(1, 2, 3) . PKA isoforms are generated by the synthesis of four types of cAMP-binding or regulatory (R) subunits that are encoded by distinct genes(4, 5) . R subunits undergo homodimerization and confer unique physical and functional properties on heterotetrameric (R(2)C(2)) PKAs that contain similar or identical catalytic (C) subunits (reviewed in (4) and (5) ). Individual PKA isoforms, which are named according to their R subunits, are thought to play specialized physiological roles at certain stages of male germ cell differentiation(1, 2, 3) . Both the temporal patterns of expression and distinct intracellular locations of R subunit isoforms are consistent with this idea. RIalpha and its cognate mRNA are expressed in premeiotic and early postmeiotic germ cells(1, 2) . Moreover, the RIalpha polypeptide persists in elongating spermatids and mature sperm. In contrast, RIIbeta mRNA and protein are initially expressed at a relatively late postmeiotic stage. As spermatocytes proceed through nuclear condensation and elongation the level of RIIbeta polypeptide declines, and this isoform is not detected in mature sperm(1, 2) . RIIalpha expression is initiated in parallel with RIIbeta accumulation. However, the level of RIIalpha polypeptide becomes maximal in late spermiogenesis, and the protein persists in mature, epididymal sperm(1, 2, 3, 6) .

Activation of PKA in mature spermatozoa elicits the initiation and maintenance of flagellar movement(7, 8) . This well established physiological response to cAMP is correlated with the cyclic nucleotide-stimulated sliding of a cytoskeletal structure (the fibrous sheath) over an internal microtubular structure called the axoneme(9) . In mature spermatozoa PKAIalpha (RIalpha(2)C(2)) is evident in the cytoplasm and plasma membrane(3) . In contrast, a high proportion of RIIalpha (and PKAIIalpha) is sequestered in the cytoskeleton. Thus, the C subunit of PKAIIalpha may catalyze selectively the phosphorylation of proximal regulatory and/or structural proteins in the cytoskeleton. These phosphoproteins may, in turn, mediate the dynamic reorganization of the flagellar cytoskeleton that is essential for motility and fertilization.

Type IIalpha and type IIbeta PKAs are often attached to the cytoskeleton or other organelles via the binding of RIIalpha or RIIbeta with A kinase anchor proteins (AKAPs) (reviewed in (10) and (11) ). AKAPs, as typified by neuronal AKAPs 75, 79, and 150(12, 13, 14) , are proteins that possess both a high affinity binding site for RIIbeta/RIIalpha and an independent domain that targets and links RII-AKAP complexes to specific intracellular sites(15) . This arrangement can place PKAIIalpha and/or PKAIIbeta in proximity with organelle-bound substrates, thereby creating a target site for cAMP action(10, 11, 12, 13, 14) . RIIalpha (PKAIIalpha) accumulates at two sites in the sperm flagellum(16) . The bulk of the RIIalpha polypeptide is attached to the outer membrane of specialized ``germ cell'' mitochondria that form a helical array around the outer dense fibers and axoneme in the ``midpiece'' of the flagellum. A lesser fraction of RIIalpha is associated with the fibrous sheath in a distal portion (the ``principal piece'') of the flagellum.

Recently, Carrera et al.(17) cloned and sequenced cDNAs encoding a major fibrous sheath protein p82. p82 binds RIIalpha and contains two short segments that share sequence similarity with the targeting domains of neuronal AKAP75(15) . It is likely that p82 mediates the binding of PKAIIalpha to the fibrous sheath.

Major questions regarding the targeting of signals carried by cAMP in germ cells remain unanswered. How is the bulk of PKAIIalpha anchored on the outside surface of mitochondria? Does an AKAP mediate this localization? If so, is a previously characterized or a novel AKAP polypeptide used? Is the anchor protein developmentally regulated and targeted principally to mitochondria?

We now describe the cloning and characterization of cDNAs that encode a unique germ cell anchor protein designated spermatid AKAP84 (S-AKAP84). S-AKAP84 contains an RII binding site and a putative mitochondrial targeting sequence. Moreover, S-AKAP84 accumulates as spermatids undergo nuclear condensation and flagellar elongation. The timing of expression of S-AKAP84 appears to be synchronized with the accumulation of RII subunits and the migration of mitochondria from the cytoplasm (round spermatids) to the cytoskeleton (midpiece in elongating spermatids). Immunofluorescence analysis documented directly that the RII binding protein is co-localized with the helical array of mitochondria in the midpiece of the flagellum.


EXPERIMENTAL PROCEDURES

Screening of cDNA Libraries

A human testis cDNA library in the expression vector gt11 (Clontech, Palo Alto, CA) was screened by the procedure of Bregman et al.(12, 13) . This method detects AKAP-beta-galactosidase fusion proteins in phage plaques by their ability to bind P-labeled RIIbeta. Two recombinant phage clones (T1 and T2) that contained overlapping cDNA sequences were purified from a population of 5 times 10^5 plaques. A 5` fragment of the larger (1.8-kilobase pair) cDNA (T1) was employed as a template to synthesize random-primed, P-labeled cDNA for further screening (see ``Results''). Eight independent cDNA clones (T3-T10) were obtained from a human testis 5` stretch (oligo(dT)- and random-primed) cDNA library in bacteriophage gt10 (Clontech) using procedures and conditions described in a previous publication(18) .

DNA Sequence Analysis

cDNA inserts from phage clones T1-T10 were cloned in the plasmid pGEM7Z (Promega) to generate the plasmid series pGT1-pGT10. DNA inserts were sequenced by the dideoxynucleotide chain termination procedure of Sanger et al.(19) as described previously(18, 20) . Sequencing reagents were obtained from U.S. Biochemical Corp.

Computer Analysis

Analyses of sequence data, sequence comparisons, and data base searches were performed using PCGENE-IntelliGenetics software (IntelliGenetics, Mountainview, CA) and the BLAST program (21) provided by the NCBI server at the National Library of Medicine/National Institutes of Health.

Expression and Purification of a Partial S-AKAP84 Polypeptide

A DNA insert that encodes amino acids 193-357 in S-AKAP84 was amplified via the Taq DNA polymerase chain reaction(15) . The 5` primer (5`-CTGACATATGGGGGAGAGGGGAAGAGAGA-3`) contained an ATG codon in the context of an NdeI restriction site and 19 downstream nucleotides that match nucleotides 639-657 in the S-AKAP84 cDNA sequence. The 3` primer (5`-ATCGGGATCCTCATCTGAGATCACTTGGGAGAT-3`) introduced a 3` BamHI recognition site and a translation termination codon after nucleotide 1135. The last 20 nucleotides of the 3` primer complement nucleotides 1116-1135 of S-AKAP84 cDNA (Fig. 1A). Amplified cDNA was digested with NdeI and BamHI and cloned into the expression plasmid pET14b (Novagen), which was cleaved with the same restriction endonucleases.


Figure 1: cDNA and derived amino acid sequences for S-AKAP84. A, numbering for the nucleotide sequence is presented on the right; amino acid residue positions are indicated on the left. Panel B shows the locations and sequences of the candidate mitochondrial signal/anchor domain, the potential leucine zipper region, and the predicted RIIbeta/RIIalpha binding site.



In recombinant pET14b, the partial S-AKAP84 cDNA is preceded by plasmid DNA that encodes an initiator ATG and 19 additional amino acids (including 6 consecutive His residues). Transcription of the chimeric gene is governed by a promoter sequence for bacteriophage T7 RNA polymerase. The partial S-AKAP84 protein (designated P21 in accord with its calculated M(r) of 21,000) was expressed in Escherichia coli BL21 (DE3) and purified to near homogeneity by metal-chelate affinity chromatography as described by Li and Rubin(22) . A 500-ml culture of bacteria yielded 2 mg of P21.

Production and Purification of Antibodies Directed against S-AKAP84

Anti-P21 serum was obtained as described previously (23) . IgGs directed against S-AKAP84 were purified from 4 ml of serum by affinity chromatography on a 2-ml column of P21-Sepharose 6B (1.7 mg P21/ml resin) as described in Land et al.(23) .

Deletion Mutagenesis of S-AKAP84

Deletion mutagenesis was performed via the polymerase chain reaction as described for AKAP75 (15) . The strategy described above for generating P21 illustrates the approach. Each 5` primer (5`-CTGACATATGN-3`) introduced an ATG codon in the context of an NdeI restriction site. This sequence preceded 21 nucleotides that encode the first 7 residues at the NH(2) terminus of the truncated protein. Each 3` primer (5`-ATCGGGATCCTCAN-3`) contained a 3` terminal BamHI site and created a stop codon after the desired COOH-terminal residue. The remaining 21 nucleotides in the 3` primer complement the last 7 codons at the COOH terminus of the truncated protein. Mutants were verified by DNA sequencing. Amplified cDNAs were cloned into pET14b, and truncated proteins were expressed in E. coli BL21 (DE3) as described by Li and Rubin (22) . Table 1gives the nomenclature for the truncated proteins and indicates the segment of S-AKAP84 that was expressed in bacteria.



Isolation and Fractionation of Germ Cells

A mixture of pachytene spermatocytes, round spermatids, and spermatids undergoing tail elongation and nuclear condensation (i.e. ``condensing'' spermatids) was obtained by sequentially incubating decapsulated adult mouse testes with collagenase and trypsin/DNase I, as described by Romrell et al.(24) and Bellve et al.(25) . Purified populations of each cell type were isolated by sedimenting the cell mixture (at unit gravity) through a 2-4% (w/v) gradient of albumin in Krebs-Ringer bicarbonate medium(17) . Spermatozoa were obtained from the cauda epididymides. Cytosolic and particulate fractions of mouse testis were prepared as described previously(13) .

Electrophoresis of Proteins

Samples of cells, cell fractions, or purified proteins were denatured in gel loading buffer and subjected to electrophoresis in polyacrylamide gels containing 0.1% SDS as described previously(12) . Western blots were prepared by transferring the size-fractionated polypeptides and molecular weight standards to an Immobilon P (polyvinylidene difluoride) membrane (Millipore Corp.), as described in Bregman et al.(12) .

Assay for RIIbeta Binding Activity

Western blots were probed with 0.3 nMP-labeled RIIbeta (2 times 10^5 cpm P radioactivity/ml), and RIIbeta binding proteins were visualized by autoradiography as indicated in several papers(12, 13, 15) . Results were quantified by scanning and integrating with a PhosphorImager (Molecular Dynamics) coupled to a computer running ImageQuant software (Molecular Dynamics).

Western Immunoblot Assays

Western blots of proteins from fractionated germ cells and testis were blocked, incubated with antiserum (1:1000) or affinity-purified anti-S-AKAP84 IgGs (1:1000 relative to serum), and washed as described previously(15, 26) . S-AKAP84 and partial S-AKAP84 polypeptides were visualized by indirect chemiluminescence using an ECL kit from Amersham Corp. as previously reported(26, 27) . Relative amounts of antigen were determined by scanning densitometry (Molecular Dynamics) of chemiluminescence signals on x-ray film. Standard curves were prepared with 0.5-100 ng of purified S-AKAP84. Amounts of S-AKAP84 protein in experimental samples were obtained from the linear portion of the standard curve.

Northern Gel Analysis

Total RNA was isolated from purified germ cells and mouse testis as described by Carrera et al.(17) . RNAs were fractionated by electrophoresis in a denaturing agarose gel, transferred to nitrocellulose, and probed with P-labeled cDNA (10^6 cpm/ml), corresponding to nucleotides 762-1260 in the S-AKAP84 sequence (Fig. 1A) as described previously(17) . Signals were visualized by autoradiography.

A multiple-tissue RNA blot containing size-fractionated human poly(A) RNAs (2 µg/lane) was obtained from Clontech. The blot was probed with the P-labeled cDNA described above. Hybridization, washing, and autoradiography were performed as described previously(28) .

Immunofluorescence Microscopy

A mixed germ cell population was prepared by mincing testis with a razor blade and then gently pipetting to release cells from the seminiferous tubules. Germ cells were fixed and permeabilized as described by Carrera et al.(17) . The specimens then were incubated sequentially with affinity-purified anti-S-AKAP84 IgGs (1:100 relative to serum) and fluorescein-conjugated anti-rabbit IgG secondary antibodies (1:100). As a control for specificity of binding, the antibody (1:100) was preabsorbed with P21 fusion protein (2 µg) for 2 h at room temperature prior to its incubation with the germ cells. The intracellular localization of the anchor protein was observed in a Zeiss Photomicroscope III equipped with epifluorescence and was photographed with Kodak T-Max P3200 film.


RESULTS

Cloning and Sequence Analysis of cDNAs Encoding a Novel AKAP

A human testis cDNA library in bacteriophage gt11 was screened for the expression of beta-galactosidase fusion proteins that bind P-labeled RIIbeta with high affinity. Two positive recombinant phage clones (T1 and T2) were purified to homogeneity. The cDNA inserts from T1 and T2 were subcloned into the EcoRI site of pGEM7Z and sequenced. The larger T1 cDNA insert included the cDNA sequence from T2 and began with an open reading frame for 401 amino acids. The coding region was followed by a translation termination signal and >500 base pairs of 3` untranslated sequence. These observations and the absence of a consensus initiator ATG indicated that the cDNAs were incomplete and lacked upstream coding and 5`-untranslated sequences.

Subsequently, a 499-base pair ApaI fragment, corresponding to nucleotides 123-621 at the 5` end of the T1 cDNA, was used to generate P-labeled cDNA for further screening. A human testis cDNA library enriched in 5` sequences yielded eight cDNA clones that were analyzed by sequencing. The cDNA designated pGT7 contained novel 5`-coding and 5`-untranslated sequences linked to the complete downstream coding and untranslated sequences determined for T1 cDNA. The remaining phage clones contained overlapping partial cDNA sequences that were identical to portions of the cDNAs in pGT7 and T1. The net result from multiple rounds of analysis is that each segment of the testis AKAP cDNA was sequenced from both strands in at least three independent cDNA clones. The data are presented in Fig. 1A.

An open reading frame of 1779 base pairs begins at an initiator ATG (nucleotides 63-65) that lies within a consensus translation start site(29) . Although the exact size of the 5`-untranslated region is unknown, the occurrence of an in-frame translation stop codon at nucleotides 42-44 precludes the possible utilization of a distal, upstream initiator ATG. The AKAP open reading frame terminates with a stop codon at nucleotides 1842-1844 (Fig. 1A). The sequence of >500 base pairs of 3`-untranslated sequence was determined, but neither a poly(A) tail nor a polyadenylation signal was evident. Since a 3.2-kb mRNA hybridized with the newly cloned cDNA (see Fig. 4), it is possible that the total length of the 3`-untranslated region exceeds 1.2 kb. However, the length and complete sequence of the 5`-untranslated region also remain to be determined.


Figure 4: Size and abundance of S-AKAP84 mRNA in human tissues. A Northern blot, which contained 2 µg of size-fractionated poly(A) RNA in each lane, was probed with P-labeled S-AKAP84 cDNA corresponding to nucleotides 762-1260 in Fig. 1A (see ``Experimental Procedures''). The source of the poly(A) RNA is indicated at the top of each lane. The gel was calibrated by running an RNA ladder in a parallel lane and staining with ethidium bromide. The sizes of the major S-AKAP84 mRNA in testis and the minor S-AKAP84 transcript in other tissues are indicated. An autoradiogram is shown.



Nomenclature and Structural Features of the S-AKAP84 Polypeptide

The protein encoded by the cDNA sequence shown in Fig. 1A is named spermatid-A kinase anchor protein 84 or S-AKAP84 because it (a) binds RIIbeta and RIIalpha, (b) exhibits an apparent M(r) of 84,000 upon electrophoresis in an SDS-polyacrylamide gel, and (c) is expressed in male germ cells. Experiments documenting these properties are presented below.

The open reading frame in Fig. 1A reveals that S-AKAP84 comprises 593 amino acids and has a calculated M(r) of 62,912. The amino acid composition of S-AKAP84 is atypical; the protein is enriched in Glu, Pro, and Ser, which account for 31% of the residues in the predicted sequence. The abundance of Glu residues is reflected in the predicted isoelectric point (pI = 4.55) and net charge(-36) of the polypeptide at pH 7.4.

The sequence of S-AKAP84 is not homologous with protein sequences compiled in the SWISS-PROT, GenBank, and PIR data bases. However, the novel protein includes two short motifs that may correspond to functional domains. Four tandem repeats of the heptapeptide consensus sequence DRNEEGL are evident between amino acid residues 310 and 338 (Fig. 1A). The beginning and end of the reiterated region are closely bordered by the tripeptide NEE (residues 306-308 and 341-343), which corresponds to the central core of the consensus heptapeptide. The occurrence of a Leu residue at the seventh position in each repeated unit raises the possibility that this segment of S-AKAP84 constitutes a coiled-coil or leucine zipper region(30) . Leucine zipper regions often mediate the homo- and/or hetero-oligomerization of protein subunits. An important caveat is that the heptapeptide repeats of S-AKAP84 lack an internal hydrophobic residue that is conserved in prototypical leucine zipper domains(30, 31) .

A lengthy hydrophobic region (amino acid residues 8-26, Fig. 1A) is evident near the NH(2) terminus of S-AKAP84. The hydrophobic domain and contiguous NH(2)- and COOH-terminal flanking sequences were compared with classical ``signal sequences'' via computer programs (32, 33) . The results suggest that this portion of S-AKAP84 does not constitute a classical signal sequence capable of targeting the protein to a secretory pathway or the plasma membrane. Instead, aspects of the organization and properties of the NH(2) terminus of S-AKAP84 match more closely with features described for the NH(2)-terminal segment of NADH-cytochrome b(5) reductase(34, 35) . The key shared properties in S-AKAP84 are as follows: (a) the first 7 residues include basic and hydroxylated amino acids (Arg^6, Ser^7); (b) a long, extremely hydrophobic segment (19 residues) provides a contiguous stop-transfer/hydrophobic anchor domain; (c) positively charged downstream residues (Arg, Lys, Lys, His, His; Fig. 1A) complete and stabilize the stop transfer signal; and (d) acidic residues are excluded from the NH(2) terminus and first appear 10 residues downstream from the end of the hydrophobic segment. Similar features target the NH(2) terminus of NADH-cytochrome b(5) reductase to the outer membrane of mitochondria(35) . The stable, post-translational insertion of the anchor sequence in the outer membrane tethers this enzyme at a physiologically relevant location and simultaneously ensures that its catalytic domain is exposed in the cytoplasm. Locations and sequences of potentially important structural motifs in the S-AKAP84 polypeptide are shown in Fig. 1B.

Preparation and Specificity of Anti-S-AKAP84 IgGs

P21, a fusion protein antigen that contains amino acids 193-357 of S-AKAP84 (see ``Experimental Procedures''), was injected into rabbits to obtain antiserum. IgGs directed against S-AKAP84 were isolated by affinity chromatography on P21-Sepharose 6B. The purified IgGs avidly bound both P21 (Fig. 2A, lane 1) and an 84-kDa protein from mouse testis (Fig. 2B, lane 1). The antibodies also produced weak signals with a 120-kDa polypeptide (Fig. 7B, and see below) and two smaller proteins (Fig. 2B, lane 1 and Fig. 7B). The latter proteins were observed only occasionally and appear to be proteolytic fragments of the 84-kDa anchor protein. Binding of anti-S-AKAP84 IgGs to target antigens was inhibited when antibodies were preincubated with excess recombinant P21 (Fig. 2A, lane 2 and Fig. 2B, lane 2). Anti-S-AKAP84 IgGs produced a detectable chemiluminescence signal with as little as 0.1 ng of purified recombinant P21 (data not shown). Thus, the antibodies are selective and sensitive.


Figure 2: Characterization of antibodies directed against S-AKAP84. Western blots were prepared as described under ``Experimental Procedures.'' A, lanes 1 and 2 were loaded with 30 ng of purified P21 fusion protein; B, lanes 1 and 2 received 30 µg of particulate proteins from mouse testis. The membranes were probed with affinity-purified anti-S-AKAP84 IgGs (1:1000) as described under ``Experimental Procedures.'' Purified P21 (1 µg/ml) was included in the buffer when membranes containing the proteins fractionated in lane 2, (A) and lane 2 (B) were incubated with affinity-purified IgGs. The immunoblots were developed by the enhanced chemiluminescence procedure, and the signals were recorded on x-ray film. The weakly immunoreactive proteins (120 kDa and <84 kDa in testis (B, lane 1) are more evident in Fig. 7B, lane 5 (see below), where twice as much protein was analyzed and the time of exposure to x-ray film was increased by a factor of 2.5.




Figure 7: Expression and RII binding activity of S-AKAP84 in fractionated germ cells and testis. Samples of total protein (30 µg) from pachytene spermatocytes (lane 1), round spermatids (lane 2), condensing spermatids (lane 3), and mature sperm (lane 4) and an aliquot of the particulate fraction (60 µg) of an adult testis homogenate (lane 5) were subjected to electrophoresis in a 0.1% SDS, 8.5% polyacrylamide gel (see ``Experimental Procedures''). After transfer to Immobilon P membranes, the size-fractionated proteins were probed with P-labeled RIIbeta (A) or affinity-purified antibodies directed against S-AKAP84 (A) as indicated under ``Experimental Procedures.'' The chemiluminescence signals in B are proportional to the amount of binding protein expressed; the autoradiogram in A shows the RIIbeta binding activity. Only the relevant portions of the gels are shown. S-AKAP84 was not present in testis cytosol. When a replicate Western blot was probed with antibodies that were preincubated with excess recombinant S-AKAP84 or P21, no signals were obtained.



An RII Binding Site Lies between Residues 331 and 389 in the S-AKAP84 Polypeptide

A combination of deletion mutagenesis and expression of partial S-AKAP84 polypeptides in E. coli was used to map the RII binding region. The ability of wild type and truncated S-AKAP-84 proteins to bind P-labeled RIIbeta was monitored by an ``overlay binding assay''(13, 15, 22) . (S-AKAP84 also binds RIIalpha avidly, (^2)but studies described in this paper were performed with RIIbeta. RI subunits are not bound by S-AKAP84).^2 Amounts of full-length and partial AKAP polypeptides synthesized were independently assessed by Western immunoblot analysis.

Partial S-AKAP84 proteins were generated by NH(2)- and/or COOH-terminal truncation as indicated in Table 1. Signals indicating expression levels and RIIbeta binding activities for a representative subset of mutant proteins are shown in Fig. 3. Deletions of 200 amino acids from the COOH and NH(2) termini of S-AKAP84 did not markedly alter specific RIIbeta binding activity (i.e. binding of P-labeled ligand/mol of expressed protein) (Fig. 3A, lanes 1-7). However, when residues 358-389 were eliminated, binding activity was extinguished (Fig. 3A, lane 8). The absence of RIIbeta binding activity in a partial S-AKAP84 protein that contains residues 358-593 (Fig. 3A, lane 9) suggested that Glu and adjacent NH(2)-terminal residues (Fig. 1A) constitute a portion of the RIIbeta tethering domain. Inspection of residues 355-376 in the S-AKAP84 sequence revealed that the positions of branched aliphatic side chains (VIX(6)VLX(3)VX(3)AX(2)VC) can be aligned in register with bulky aliphatic residues that mediate the high affinity binding of RIIbeta by neuronal AKAP75 (LLX(6)LVX(3)IX(3)IX(2)LV) (15) . The RIIbeta tethering site in AKAP75 comprises amino acids 392-413 and functions as an independent domain(15) . Only one potentially significant difference is noted in the comparison. The occurrence of Ala in S-AKAP84 conserves the hydrophobic character and alpha-helix-forming propensity of Ile in AKAP75, but the methyl side chain contributes a smaller apolar surface. Substitution of branched chain amino acids with Ala diminishes the avidity of AKAP75 for RIIbeta. However, the presence of neighboring Val in S-AKAP84 may compensate for this deficiency.


Figure 3: Expression and RIIbeta binding activity of truncated S-AKAP84 polypeptides. Deletion mutants of S-AKAP84 were expressed in E. coli BL21 as described under ``Experimental Procedures.'' Samples (0.5 µg of total protein; 20-50 ng of recombinant protein) of the soluble fraction of bacterial lysates were subjected to electrophoresis in a 0.1% SDS, 10% polyacrylamide gel. After transfer to Immobilon P membranes, the size-fractionated proteins were probed with P-labeled RIIbeta (A) or antibodies directed against S-AKAP84 (B) as described under ``Experimental Procedures.'' The densitometric quantification of wild type and mutant S-AKAP84 proteins by antibody binding was used to normalize for variations in the levels of recombinant protein expression. The autoradiogram in panel A shows RIIbeta binding activities; the chemiluminescence signals in panel B are proportional to the amounts of the binding proteins. The nomenclature for recombinant wild type and mutant RIIbeta binding proteins is given in Table 1. Lanes 1-9 received extracts from E. coli expressing the Delta0, DeltaN115, DeltaN190, DeltaN190-DeltaC97, DeltaN190-DeltaC151, DeltaN190-DeltaC177, DeltaN190-DeltaC204, DeltaN190-DeltaC235, and DeltaN358 proteins, respectively. The recombinant protein in lane 9 was visualized by staining a parallel lane loaded with 5 µg of total protein because the epitopes bound by anti-S-AKAP84 IgGs were deleted. Calculated M(r) values for the various polypeptides are indicated. Only the relevant regions of the autoradiograms are shown. E. coli extracts that contained the DeltaN34 and DeltaN190-DeltaC124 proteins (see Table 1) yielded signals that were similar to those observed for lanes 1-7; DeltaN358-DeltaC97 did not bind RIIbeta (not shown).



Based on the preceding considerations a truncated S-AKAP84 protein that corresponds to amino acids 331-443 was expressed in E. coli. Twenty-four residues that precede the putative RII binding site were retained because (a) this region is flanked by a long NH(2)-terminal segment in wild-type S-AKAP84 and (b) there is no precedent for an RII binding domain that is congruent with the NH(2) terminus of an AKAP (10, 11, 12, 13, 14, 15) . The RIIbeta binding activity of this mutant was similar to that observed for S-AKAP84 and partial S-AKAP84 proteins in lanes 1-7 of Fig. 3A. Thus, amino acid residues that govern RII binding activity in S-AKAP84 lie between residues 331 and 389.

Determination of the Size and Relative Abundance of S-AKAP84 mRNA in Various Tissues

A Northern blot containing poly(A) RNA from several human tissues was probed with P-labeled S-AKAP84 cDNA. A 3.2-kb mRNA from testis yielded an intense hybridization signal (Fig. 4). In contrast, moderate to low levels of a 4.3-kb mRNA were detected in each of the other tissues. A low level of the 4.3-kb transcript is also present in testis. When the blot was exposed 4 times longer (48 h) a minor 7.5-kb mRNA was observed (data not shown). Moderate to low levels of the 4.3-kb and 7.5-kb transcripts were also observed in RNA samples derived from kidney, pancreas, liver, lung, and brain.

Since Southern blots containing restriction enzyme digests of human genomic DNA yield a simple pattern that is consistent with a single-copy gene (data not shown), the Northern analysis suggests that S-AKAP84 RNA transcripts undergo alternative splicing. If multiple promoters drive transcription of the S-AKAP84 gene, they could also contribute to the diversity of transcripts. The smaller S-AKAP84 mRNA is expressed exclusively in testis (Fig. 4). PhosphorImager analysis disclosed that the testis-specific 3.2-kb mRNA is 10-100-fold more abundant than the 4.3-kb S-AKAP84 mRNA expressed in other tissues.

Accumulation of S-AKAP84 mRNA and Expression of the Cognate Anchor Protein Are Late Events in Postmeiotic Spermatogenic Development

In order to investigate the developmental regulation of S-AKAP84 expression, studies were performed on the mouse model system. Human S-AKAP84 cDNA hybridized strongly with a 3.2-kb mRNA from mouse germ cells. ( Fig. 5and 6). This mRNA encodes a murine RIIbeta binding protein that is homologous with human S-AKAP84. (^3)Murine S-AKAP84 mRNA was not detected in the population of total testis poly(A) RNAs during early postnatal and juvenile development (Fig. 5). The transcript is not evident even when postmeiotic round spermatids are present (days 20 and 24; Fig. 5). However, a substantial level of S-AKAP84 mRNA accumulates as the animals gain the capacity to reproduce (Fig. 5, lane A).


Figure 5: Expression of S-AKAP84 mRNA in the testes of mice of various ages. Total testis RNA was isolated from mice of the indicated ages as described by Carrera et al.(17) . The adult animals (A) were 10 weeks old. Samples of RNA (20 µg) were fractionated by electrophoresis under denaturing conditions and transferred to nitrocellulose as described under ``Experimental Procedures.'' The Northern blot was probed and calibrated as described in ``Experimental Procedures'' and Fig. 4. The size of the S-AKAP84 transcript is indicated. An autoradiogram is shown.



The expression pattern is consistent with the appearance of S-AKAP84 mRNA during a late phase of spermatid development. This possibility was addressed by monitoring the expression of S-AKAP84 and its cognate mRNA in purified populations of developing germ cells that correspond to meiotic pachytene spermatocytes, postmeiotic round spermatids, condensing spermatids (which undergo nuclear condensation and assume the elongated morphology of mature sperm), and epididymal sperm. S-AKAP84 mRNA was not detected in either pachytene spermatocytes or round spermatids (Fig. 6, lanes 2 and 3). In contrast, the 3.2-kb S-AKAP84 transcript is clearly evident in an enriched population of condensing/elongating spermatids (Fig. 6, lane 4). S-AKAP84 mRNA is not retained in mature sperm. The expression pattern of an 84-kDa RIIbeta binding protein parallels the developmentally controlled accumulation and disappearance of S-AKAP84 mRNA (Fig. 7A). A candidate 84-kDa anchor protein is also independently identified by its avid binding with affinity-purified anti-S-AKAP84 IgGs (Fig. 7B, lane 3). Moreover, the binding assay and antibodies reveal an 84-kDa polypeptide that corresponds to a major RIIbeta binding protein in the particulate fraction of testis homogenates (Fig. 7, A, lane 5, and B, lane 5). The highly sensitive immunoblot-chemiluminescence assay (see above) reveals a low level of the 84-kDa protein in round spermatids (Fig. 7B, lane 2). The lack of signals for S-AKAP84 mRNA (Fig. 6, lane 3) and RII binding activity (Fig. 7A, lane 2) in the round spermatid population may reflect lower levels of sensitivity inherent in these measurements. It is also possible that the 84-kDa protein in round spermatids fails to bind RIIbeta because its tethering function is modulated by developmental stage-specific, post-translational modification. Overall, more than 90% of S-AKAP84 immunoreactivity is associated with condensing/elongating spermatids. (^4)


Figure 6: Expression of S-AKAP84 mRNA in fractionated germ cells. Total RNA (20 µg/lane) from spleen (a negative control, lane 1), pachytene spermatocytes (lane 2), round spermatids (lane 3), and condensing spermatids (lane 4) were subjected to Northern gel analysis as described in the legend to Fig. 5and under ``Experimental Procedures.'' An autoradiogram is presented, and the size of S-AKAP84 mRNA is indicated.



The apparent M(r) of the murine RIIbeta binding protein is estimated to be 84,000 when it is compared with protein standards. Proteins of similar size are observed when extracts of rat, human, and bovine testis are subjected to RIIbeta binding and immunoblot analyses.^2 Other tissues do not contain the 84-kDa protein. The discrepancy between the calculated M(r) (63,000) and the apparent M(r) is probably due to the highly acidic and Pro-rich nature of the protein (Fig. 1A). Proteins with these properties often bind SDS poorly and assume atypical conformations under denaturing conditions. Other AKAPs exhibit similar properties and have aberrantly large apparent M(r) values(10, 26) .

A very low level of a 120-kDa protein is also evident in testis and fractionated germ cells (Fig. 7B, lanes 2, 3, and 5). This protein (917 residues) is encoded by a 3.1-kb, alternatively spliced S-AKAP84 mRNA.^3 Structure/function analysis of the 120-kDa protein is in progress.

S-AKAP84 Is Targeted to Mitochondria in the Midpiece of Condensing Spermatids

The intracellular location of S-AKAP84 was established by immunofluorescence microscopy. When a mixed population of developing germ cells was probed with antibodies directed against S-AKAP84 only condensing spermatids (Fig. 8) and their developmental by-product, anucleate residual bodies (not shown), emitted intense fluorescence signals. The fluorescence signal from condensing spermatids was precisely congruent with the previously described (36) coil of 70-80 mitochondria that form a helical array in the midpiece (Fig. 8). Staining was excluded from the head, the tail, and the remainder of the flagellum including the axoneme, the fibrous sheath, the outer dense fibers, and the plasma membrane. Thus, S-AKAP84 accumulates de novo in a late stage of spermatogenesis. In addition, this anchor protein is targeted selectively to the major RII binding site in murine spermatozoa, the mitochondrial sheath of the midpiece region.


Figure 8: S-AKAP84 is targeted selectively to the mitochondrial sheath. A representative example of a late condensing spermatid is presented. The phase contrast photograph (A) shows the characteristic morphology of the head containing the condensed nucleus, the midpiece with its characteristic ``corkscrew'' (helical) structure and the thinner principal piece. B, when the sample was probed with anti-S-AKAP84 IgGs and a fluorescein-conjugated secondary antibody, an intense fluorescence signal was obtained from the helical array of mitochondria in the midpiece. No comparable staining was observed for germ cells at any other stage of development. The signal observed in panel B was eliminated by preincubating the antibodies with an excess of the partial S-AKAP84 polypeptide antigen P21.




DISCUSSION

A cDNA encoding a novel, spermatid AKAP (S-AKAP84) has been cloned and characterized. Previous investigations documented that PKAIIalpha is associated with two distinct components of the spermatozoan cytoskeleton: the fibrous sheath in the principal piece and the outer membranes of an array of mitochondria located in the midpiece(16) . Most of the RIIalpha subunits are sequestered by the mitochondria. Recently, Carrera et al.(17) demonstrated that an abundant cytoskeletal protein, p82, mediates the anchoring of RII (PKAII) in the fibrous sheath. Experiments described herein strongly implicate S-AKAP84 in the delivery (targeting) of RII (PKAII) to the midpiece. The NH(2) terminus of S-AKAP84 has several structural features that parallel the properties of signal/anchor domains (see ``Results''). Such domains target NADH-cytochrome b(5) reductase and several other proteins to the outer mitochondrial membrane(35) . The properties of the NH(2)-terminal segment of S-AKAP84 (residues 1-30) are consistent with the location of the protein in situ. Immunofluorescence microscopy demonstrated that S-AKAP84 is targeted selectively to a large, helical structure in the midpiece of spermatids undergoing nuclear condensation and tail elongation (Fig. 8). The helical suprastructure corresponds to a precisely arranged assembly of 70-80 mitochondria, otherwise known as the mitochondrial sheath(36) . Thus, S-AKAP84 accumulates in a flagellar compartment that also contains a high proportion of the anchored RIIalpha (PKIIalpha) in mature spermatozoa(3, 6, 16) . The highly specialized germ cell mitochondria are components of the midpiece cytoskeleton. In late postmeiotic stages of spermatogenesis, a portion of the outer membrane of each mitochondrion closely apposes the outer dense fibers (another cytoskeletal structure), whereas the remaining mitochondrial surface directly contacts the cytoplasm.

The putative signal/anchor domain of S-AKAP84 is predicted to insert into the outer membrane bilayer post-translationally(35) . Thus, all other functional domains in organelle-sequestered S-AKAP84 molecules would be concentrated in a thin layer of cytoplasm adjacent to the mitochondrial surface. Therefore, the RII binding region located between residues 331 and 389 in S-AKAP84 would be accessible to mediate the tethering of cytoplasmic PKAII isoforms. PKAII captured by this mechanism could control or modulate flagellar activities by phosphorylating co-localized target substrates in the cytoskeleton, thereby altering their functional and/or structural properties.

The sequence of S-AKAP84 diverges markedly from the primary structures of all other AKAPs, with the exception of one short but potentially important domain. A 22-residue segment of the RII binding region of S-AKAP84 (amino acids 355-376) contains a group of hydrophobic, branched chain amino acids that align precisely with Ile, Leu, or Val residues in the 22-amino acid sequence that constitutes the RIIbeta binding domain of the neuronal AKAP, AKAP75(15) . Moreover, truncated S-AKAP84 polypeptides that lack residues 355-358 or 359-376 have no RII binding activity (Fig. 3, and ``Results''). Since (a) the long, aliphatic side chains in the tethering domain of AKAP75 are essential for high affinity RII binding activity and (b) similar patterns of hydrophobic, aliphatic side chains are evident in non-neuronal AKAPs(10, 11) , it appears that the sequence encompassed by residues 355-376 in S-AKAP84 may constitute a tethering site. The inclusion of a 20-22-residue module that conserves the spacing among long aliphatic side chains (and presumably a precise orientation of hydrophobic surfaces in a higher order structure) in otherwise divergent proteins, provides a mechanism for targeting PKAII isoforms to a diverse array of intracellular target sites (see Refs. 10 and 11).

Overall, the properties of S-AKAP84 fulfill criteria that are used in establishing the physiological significance of an anchor protein. The polypeptide contains structural features that appear to account for both the sequestration of RII and the targeting/anchoring of AKAP-RII (or PKAII) complexes at a previously established target site for cAMP action. Further experiments, involving site-directed mutagenesis and transfection/expression analysis, will be required to (a) verify the proposed roles of the NH(2)-terminal targeting and centrally located tethering domains of S-AKAP84 and (b) elucidate the exact roles of individual amino acids in each functional domain.

The pattern of the developmental regulation of S-AKAP84 expression is quite atypical and provides additional, albeit indirect, clues regarding the function of the anchor protein. The RII binding protein and its cognate mRNA are apparently expressed de novo during late spermiogenesis (Fig. 5Fig. 6Fig. 7). Since the transcription of most germ cell genes is silenced at or before this stage of development (37) , the data suggest that S-AKAP84 subserves a ``late'' developing, cAMP-mediated signaling pathway that emerges with temporal precision. Furthermore, S-AKAP84 accumulation occurs as the RIIalpha and RIIbeta polypeptides reach their maximal levels (1, 2) and in parallel with the remodeling and reorganization of spermatid mitochondria(36) . In the latter instance, classically shaped mitochondria are dispersed in the cytoplasm of round spermatids; as the cells undergo nuclear condensation and tail elongation the mitochondria migrate to the outer dense fibers of the midpiece cytoskeleton and assume a crescent shape (36) . These mitochondria align end-to-end to form a helical array. It is thought that preexisting mitochondria are modified by the insertion of novel proteins during this period of transformation. Our results indicate that S-AKAP84 and possibly S-AKAP84 complexed with PKAII are incorporated into the outer mitochondrial membrane during this major developmental transition. These observations raise the possibility that S-AKAP84-PKAII complexes play a crucial role in initiating or modulating this key step in sperm development. Ultimately, it will be necessary to disrupt the S-AKAP84 gene or otherwise compromise S-AKAP84 expression to establish the exact physiological role of the anchor protein.

A puzzling aspect of the results is that S-AKAP84 is not detected in mature mouse sperm. In contrast, the association of RIIalpha with the mitochondrial sheath has been documented by electron microscopy in mature bovine sperm(16) . Several possible explanations may account for this apparent discrepancy. Murine S-AKAP84 may be labile and subject to artifactual degradation during the preparation of murine spermatozoa. Another possibility is that S-AKAP84 plays a central physiological role only in condensing spermatids and its vestigial retention in mature sperm is species-specific and not physiologically relevant. Alternatively, S-AKAP84 may target and deliver PKAII to the outer mitochondrial membrane, whereupon the kinase is exchanged to a second, more stable mitochondrial protein that permanently anchors the enzyme. A 105-kDa protein that might fulfill this role was detected (via a low intensity signal) in epididymal sperm (Fig. 7A, lane 4). This protein does not contain epitopes recognized by anti-S-AKAP84 IgGs (Fig. 7B, lane 4). The intracellular location and significance of the low level RII binding activity associated with the 105-kDa protein remain to be investigated. Irrespective of whether S-AKAP84 functions only in condensing spermatids or over a broader span of development, it represents the first example of a developmentally regulated, mitochondrially targeted RII anchor protein.


FOOTNOTES

*
This work was supported in part by National Institutes of Health Grant GM22792 (to C. S. R.) and U.S. Department of Agriculture Grant 92-37205-8050 (to S. B. M.) The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

The nucleotide sequence(s) reported in this paper has been submitted to the GenBank(TM)/EMBL Data Bank with accession number(s) U34074[GenBank].

(^1)
The abbreviations used are: PKA, protein kinase A (cAMP-dependent protein kinase); R, regulatory subunit of cAMP-dependent protein kinase; C, catalytic subunit of cAMP-dependent protein kinase; AKAP, protein kinase A anchor protein; kb, kilobase(s).

(^2)
R. Y. Lin and C. S. Rubin, unpublished observations.

(^3)
Q. Chen, R. Y. Lin, and C. S. Rubin, unpublished observations.

(^4)
The fibrous sheath AKAP designated p82 (17) is not bound by anti-S-AKAP84 IgGs, and its binding activity is not detected under the overlay assay conditions used in the present studies.


ACKNOWLEDGEMENTS

We thank Ann Marie Alba for expert secretarial services.


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