Complete Primary Sequences of Two λ Immunoglobulin Light Chains in Myelomas with Nonamyloid (Randall-Type) Light Chain Deposition Disease
1998; Elsevier BV; Volume: 153; Issue: 1 Linguagem: Inglês
10.1016/s0002-9440(10)65573-3
ISSN1525-2191
AutoresCatherine Decourt, Guy Touchard, Jean-Louis Preud'homme, Rubén Vidal, Hélène Beaufils, Marie‐Claude Diemert, Michel Cogné,
Tópico(s)Protein Kinase Regulation and GTPase Signaling
ResumoWe herein report on the first two primary sequences (BOU and RAC) of monoclonal light chains of the λ type responsible for nonamyloid λ light chain deposition disease. Both patients were affected with severe forms of myeloma complicated with renal failure. The pathological presentation typically featured Congo red-negative deposits along tubular basement membranes but differed somewhat from the typical “Randall-type” κ light chain deposition disease: they lacked the prominent glomerulosclerosis pattern often featuring nonamyloid κ deposits and were associated with cylinders or myeloma casts. Both protein sequences were deduced from those of the corresponding complementary DNAs in the bone marrow plasma cells. For each chain, products of three independent amplifications by polymerase chain reaction were sequenced and found to be identical. BOU and RAC λ mRNAs had a normal overall structure consisting of Vλ2 segments rearranged to Jλ2Cλ2 but displayed a number of unusual features within their primary sequences. These substitutions are likely responsible for changes in light chain conformation that promote their aggregation and deposition along renal tubule basement membranes. We herein report on the first two primary sequences (BOU and RAC) of monoclonal light chains of the λ type responsible for nonamyloid λ light chain deposition disease. Both patients were affected with severe forms of myeloma complicated with renal failure. The pathological presentation typically featured Congo red-negative deposits along tubular basement membranes but differed somewhat from the typical “Randall-type” κ light chain deposition disease: they lacked the prominent glomerulosclerosis pattern often featuring nonamyloid κ deposits and were associated with cylinders or myeloma casts. Both protein sequences were deduced from those of the corresponding complementary DNAs in the bone marrow plasma cells. For each chain, products of three independent amplifications by polymerase chain reaction were sequenced and found to be identical. BOU and RAC λ mRNAs had a normal overall structure consisting of Vλ2 segments rearranged to Jλ2Cλ2 but displayed a number of unusual features within their primary sequences. These substitutions are likely responsible for changes in light chain conformation that promote their aggregation and deposition along renal tubule basement membranes. A number of diseases may result from monoclonal immunoglobulin (Ig) tissue deposition complicating malignant or benign monoclonal B cell proliferations. These diseases are characterized by multivisceral Ig-related material deposits, most often corresponding to monoclonal light chains (LCs) or LC fragments and usually predominating in the kidney. The two most frequent pathological presentations are AL-amyloidosis and nonamyloid (Randall-type) LC deposition disease (LCDD): AL-amyloidosis deposits usually predominate in the glomerular mesangium and in arteriolar walls and mostly involve λ LCs highly organized in β-pleated sheet fibrils. By contrast, LCDD deposits (mostly of the κ type) are amorphous, predominate along the outer part of basement membranes in the distal tubule and the loop of Henlé, and often associate with marked nodular glomerulosclerosis.1Preud'homme JL Morel-Maroger L Brouet JC Cerf M Mignon F Guglielmi P Seligmann M Synthesis of abnormal immunoglobulins in lymphoplasmatic disorders with visceral light chain deposition.Am J Med. 1980; 69: 703-710Abstract Full Text PDF PubMed Scopus (88) Google Scholar, 2Preud'homme JL Morel-Maroger L Brouet JC Mihaesco E Mery JP Seligmann M Synthesis of abnormal heavy and light chains in multiple myeloma with visceral deposition of monoclonal immunoglobulin.Clin Exp Immunol. 1980; 42: 545-553PubMed Google Scholar, 3Ganeval D Noël LH Preud'homme JL Droz D Grünfeld JP Light chain deposition disease: its relation with AL-type amyloidosis.Kidney Int. 1984; 26: 1-9Crossref PubMed Scopus (169) Google Scholar, 4Bellotti V Stoppini M Merlini G Zapponi MC Meloni ML Banfi G Ferri G Amino acid sequence of κ Sci, the Bence Jones protein isolated from a patient with light chain deposition disease.Biochim Biophys Acta. 1991; 1097: 177-182Crossref PubMed Scopus (30) Google Scholar, 5Cogné M Preud'homme JL Bauwens M Touchard G Aucouturier P Structure of a monoclonal κ chain of the VκIV subgroup in the kidney and plasma cells in light chain deposition disease.J Clin Invest. 1991; 87: 2186-2190Crossref PubMed Scopus (75) Google Scholar, 6Cogné M Silvain C Khamlichi AA Preud'homme JL Structurally abnormal immunoglobulins in human immunoproliferative disorders.Blood. 1992; 79: 2181-2195PubMed Google Scholar, 7Khamlichi AA Aucouturier P Silvain C Bauwens M Touchard G Preud'homme JL Nau F Cogné M Primary structure of a monoclonal κ chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1992; 87: 122-126Crossref PubMed Scopus (42) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 9Preud'homme JL Aucouturier P Touchard G Khamlichi AA Rocca A Denoroy L Cogné M Monoclonal immunoglobulin deposition disease: a review of immunoglobulin chain alterations.Int J Immunopharmacol. 1994; 16: 425-431Crossref PubMed Scopus (23) Google Scholar, 10Denoroy L Déret S Aucouturier P Overrepresentation of the VκIV subgroup in light chain deposition disease.Immunol Lett. 1994; 42: 63-66Crossref PubMed Scopus (71) Google Scholar, 11Decourt C Cogné M Rocca A Structural peculiarities of a truncated VκIII immunoglobulin light chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1996; 106: 357-361Crossref PubMed Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar, 13Gallo G Goni F Boctor F Vidal R Kumar A Stevens FJ Frangione B Ghiso J Light chain cardiomyopathy: structural analysis of the light chain tissue deposits.Am J Pathol. 1996; 148: 1397-1406PubMed Google Scholar, 14Bellotti V Stoppini M Magione PM Fornasieri A Min L Merlini G Ferri G Structural and functional characterization of three human immunoglobulin k light chains with different pathological implications.Biochim Biophys Acta. 1996; 1317: 161-167Crossref PubMed Scopus (25) Google Scholar To date, many LCs implicated in AL-amyloidosis have been described, and a large amount of sequence data has allowed the formulation of hypotheses concerning the special role of some amino acid substitutions in the process of fibril formation.15Aucouturier P Khamlichi AA Preud'homme J Bauwens M Touchard G Cogné M Complementary DNA sequence of human amyloidogenic immunoglobulin light chain precursors.Biochem J. 1992; 285: 149-152Crossref PubMed Scopus (28) Google Scholar, 16Hurle MR Helms LR Li L Chan W Wetzel R A role for destabilizing amino acid replacements in light chain amyloidosis.Proc Natl Acad Sci USA. 1994; 91: 5446-5450Crossref PubMed Scopus (329) Google Scholar, 17Stevens PW Raffen R Hanson DK Deng YL Berrios-Hammond M Westholm FA Murphy C Eulitz M Wetzel R Solomon A Schiffer M Stevens F Recombinant immunoglobulin variable domains generated from synthetic genes provide a system for in vitro characterization of light-chain amyloid proteins.Protein Sci. 1995; 4: 421-432Crossref PubMed Scopus (107) Google Scholar, 18Stevens F Myatt EA Chang C-H Westholm FA Eulitz M Weiss DT Murphy C Solomon A Schiffer M A molecular model for self-assembly of amyloid fibrils: immunoglobulin light chains.Biochemistry. 1995; 34: 10697-10702Crossref PubMed Scopus (101) Google Scholar, 19Helms LR Wetzel R Specificity of abnormal assembly in immunoglobulin light chain deposition disease and amyloidosis.J Mol Biol. 1996; 257: 77-86Crossref PubMed Scopus (97) Google Scholar, 20Schorman N Murrell JR Lipnieks JJ Benson MD Tertiary structure of an amyloid immunoglobulin light chain protein: a proposed model for amyloid fibril formation.Proc Natl Acad Sci USA. 1995; 92: 9490-9494Crossref PubMed Scopus (79) Google Scholar By contrast, only a few LCDD chains have been studied, all of the κ type,4Bellotti V Stoppini M Merlini G Zapponi MC Meloni ML Banfi G Ferri G Amino acid sequence of κ Sci, the Bence Jones protein isolated from a patient with light chain deposition disease.Biochim Biophys Acta. 1991; 1097: 177-182Crossref PubMed Scopus (30) Google Scholar, 5Cogné M Preud'homme JL Bauwens M Touchard G Aucouturier P Structure of a monoclonal κ chain of the VκIV subgroup in the kidney and plasma cells in light chain deposition disease.J Clin Invest. 1991; 87: 2186-2190Crossref PubMed Scopus (75) Google Scholar, 7Khamlichi AA Aucouturier P Silvain C Bauwens M Touchard G Preud'homme JL Nau F Cogné M Primary structure of a monoclonal κ chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1992; 87: 122-126Crossref PubMed Scopus (42) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 9Preud'homme JL Aucouturier P Touchard G Khamlichi AA Rocca A Denoroy L Cogné M Monoclonal immunoglobulin deposition disease: a review of immunoglobulin chain alterations.Int J Immunopharmacol. 1994; 16: 425-431Crossref PubMed Scopus (23) Google Scholar, 11Decourt C Cogné M Rocca A Structural peculiarities of a truncated VκIII immunoglobulin light chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1996; 106: 357-361Crossref PubMed Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar, 13Gallo G Goni F Boctor F Vidal R Kumar A Stevens FJ Frangione B Ghiso J Light chain cardiomyopathy: structural analysis of the light chain tissue deposits.Am J Pathol. 1996; 148: 1397-1406PubMed Google Scholar and the process by which LCs aggregate is still largely unknown. We herein report on the first two λ LCs (BOU andRAC) implicated in nonamyloid LCDD. BOU andRAC belonged to the Vλ2 subgroup and included Jλ2/Cλ2 segments. In both cases, the renal lesions differed somewhat from those seen in most cases of κ nonamyloid deposits, because they did not reveal prominent glomerulosclerosis. In addition, for both patients, deposits along the tubular membrane basements were accompanied by tubular lesions resembling cast myeloma. Patient BOU, a 59-year-old French man, was referred in September 1993 for renal failure with anemia (hemoglobin, 8 g/100 ml). The creatininemia was 750 μmol/L, and proteinuria was abundant (8 g/24 hours) with a predominant λ Bence-Jones protein that was also detectable in serum in small amounts. Hypo-γ-globulinemia was marked (4 g/L). A moderate microscopic hematuria was found. Bone marrow smears showed 50% plasma cells. Light microscopic examination of a kidney biopsy showed myeloma cast nephropathy. Eighteen glomeruli were normal without nodular sclerosis. The interstitium was focally infiltrated by lymphocytes and plasma cells. Congo red staining was negative. Immunofluorescence study (Figure 1A)showed linear deposits along the tubular basement membranes, which only stained for λ chain. Electron microscopic study of a renal medulla fragment was essentially normal and did not show granular osmiophilic deposits along tubular basement membranes. From October 1993 to December 1993, the patient was given nine courses of plasmapheresis and two courses of vincristine (0.4 mg) and Adriamycin (9 mg/m2) combined the first day with prednisolone (1 mg/kg), which was continued for 4 further days. Despite this treatment, hemodialysis was required, and the patient died in December 1993 with 5% leukemic plasma cells. Patient RAC, a 48-year-old Guyanese woman, was referred in September 1996 for persistent renal failure 2 months after aPlasmodium falciparum infection. The creatinine plasma level was 547 μmol/L, and there was an abundant proteinuria (7 to 9 g/24 hours) essentially consisting of monoclonal free λ chains that were also detectable in serum by immunofixation. There was no monoclonal IgD or IgE by immunofixation, and serum polyclonal Ig levels were moderately affected (9.7 g/L of IgG, 0.3 g/L of IgA, and 0.2 g/L of IgM). Bone marrow smears showed 13% dystrophic plasma cells and allowed the diagnosis of myeloma. Light microscopic examination of a kidney biopsy mainly showed severe and diffuse tubular lesions with a moderate inflammatory cell infiltrate (Figure 1B). Some tubules were lined by a flattened epithelium; other tubules were obstructed and dilated by proteic casts; some tubular basement membranes were enlarged with Congo red-negative material; nodular glomerulosclerosis was not observed. By immunofluorescence (Figure 1C), tubular basement membrane deposits only stained with anti-λ LC antibodies and not with other anti-Ig chains or anti-complement antisera. The patient was included in a protocol composed of two autologous bone marrow transplantations. One month after the first transplantation (January 1997), creatininemia dropped to 159 μmol/L and proteinuria to 0.39 g/24 hours. The second transplantation was performed in April 1997; 2 months later the serum creatinine level was 120 μmol/L and the proteinuria 0.26 g/L, without free LC detectable in the serum. However, 10 months later, a severe relapse occurred with a heavy plasma cell infiltrate in bone marrow and with high levels of free λ LC in urine. Total RNA was prepared by lysis of bone marrow cells in 4 mol/L guanidine isothiocyanate followed by centrifugation at 170,000 ×g for 18 hours on a 5.7 mol/L cesium chloride pad. Total RNA was analyzed on a 1% agarose, 1.7 mol/L formaldehyde gel in comparison with RNA from the human lymphoma cell line IARC 518 producing normal-sized κ mRNA and from the plasmacytoma cell line RPMI 8226 producing a normal-sized λ mRNA.21Leduc I Preud'homme JL Cogné M Structure and expression of the mb-1 transcript in human lymphoid cells.Clin Exp Immunol. 1992; 90: 141-146Crossref PubMed Scopus (15) Google Scholar They were transferred to nylon sheets and hybridized with either a Cκ probe, a 2.5-kbEcoRI genomic fragment containing the human Cκ exon, or a Cλ probe, a 3.5-kb EcoRI–HindIII fragment containing the human Cλ2 exon. Total RNA was used as a template for synthesizing single-stranded cDNA using reverse transcriptase and an oligodeoxythymidylic acid primer (Boehringer Mannheim, Mannheim, Germany). PCR primers were a 5′ primer corresponding to a Vλ1-Vλ2-Vλ3 consensus leader region (5′-ATGGCCKGSWYYSYTCTCCTC-3′) and a 3′ primer complementary to the consensus upstream part of the Cλ exons (5′-CTCCCGGGTAGAAGTCACT-3′). Amplification of the cDNAs by PCR was performed with Taq polymerase (Pharmacia, Uppsala, Sweden) through 35 cycles consisting of denaturation at 94°C for 30 seconds, annealing at 53°C for 30 seconds, and elongation at 72°C for 30 seconds.22Saiki RK Scharf S Faloona F Mullis KG Horn GT Erlich HA Arnheim N Enzymatic amplification of β-globin genomic sequences and restriction site analysis for diagnosis of sickle cell anemia.Science. 1985; 230: 1350-1354Crossref PubMed Scopus (6818) Google Scholar After amplification, PCR products were fractionated on 1.2% agarose gels and sequenced by the dideoxy termination method,23Sanger F Nicklen S Coulson AR DNA sequencing with chain terminating inhibitors.Proc Natl Acad Sci USA. 1977; 74: 5463-5467Crossref PubMed Scopus (52769) Google Scholar using Taq polymerase and an automated laser fluorescent DNA sequencer (Perkin-Elmer, Branchburg, NJ). Serum and urinary proteins were analyzed by conventional agarose gel zonal electrophoresis in nondenaturing conditions and by immunofixation. For patient RAC, urinary proteins were purified using diethylaminoethyl-Trisacryl chromatography in 10 mmol/L Tris, pH 8.0, on a 0 to 0.3 mol/L sodium chloride gradient, followed by a second chromatography on Sephadex G100 in 0.1 mol/L Tris-0.5 mol/L NaCl, pH 8.0. An electrophoresis in nondenaturing conditions then showed that the protein was mainly present in dimeric form. Purified urinary RAC protein (3 mg) was dissolved in 1 ml of 0.2 mol/L NH4CO3 and digested for 1 hour at 37°C with trypsin (modified, sequencing grade; EC 3.4.21.4) (Boehringer Mannheim) at an enzyme/protein ratio of 1:100 (w/w). Proteolysis was terminated by freezing and freeze-drying. The resulting peptides were separated by reverse-phase high-performance liquid chromatography using a Vydac C18 (The Separations Group, Hesperia, CA) column (218TP52; 0.21 × 25 cm) and a 60-minute 0 to 60% linear gradient of acetonitrile-water (pH 2.1) at a flow rate of 0.2 ml/min. Automated Edman degradation sequence analysis of purified peptides was carried out on a 477A protein-peptide sequencer, and the resulting phenylthiohydantoin amino acid derivatives were identified using the online 120A PTH analyzer (Applied Biosystems, Foster City, CA). Using RNA extracted from bone marrow cells in two cases of myeloma-associated LCDDs, we studied λ LC mRNAs by Northern blotting: blots hybridized with a Cλ probe gave a strong signal at the expected correct size in both cases, although hybridization with a Cκ probe yielded no signal in the lanes corresponding to myeloma samples (Figure 2). These hybridization data indicated that the B cell population in both bone marrow samples mainly corresponded to the monoclonal λ-producing cells. In both cases, three independent reverse transcription-PCR amplifications were performed, and direct sequencing of PCR products yielded identical nucleotide sequences for all three independent amplification experiments. In addition, protein sequence analysis of urinary RAC tryptic peptides allowed the identification of peptide sequences (+9→+21, +45→+60, +66→+88, and +156→+166), which fell in complete agreement with the protein sequence deduced fromRAC cDNA. From BOU and RAC cDNA nucleotide sequences, we could deduce complete amino acid sequences and assign both LCs to the Vλ2 subgroup. In both cases, the V region was normally rearranged to the Jλ2Cλ2 segment, which did not present any sequence abnormality. On the contrary, comparison of Vλ sequences with previously reported λ chains pointed out several unusual features consisting of the appearance of residues never or rarely found at these positions (Figure 3). In protein BOU, several substitutions unique among Vλ2 proteins were noticed: Ser+2→Ala, Val+27F→Leu, Leu+46→Ile, Ile+48→Leu, Ser+65→Phe, Ser/Cys+89→Gly, Ser+90→Leu, Ala+92→Val, Ser/Asn+95→Arg, and Thr95A→Leu. Some other substitutions have been rarely observed among Vλ2 proteins: Ala+43→ Val and Thr+70→ Ala. Two other rare substitutions were encoded at the VJ junction (Val+96→Trp) and within Jλ2 (Lys103→Arg). Another feature of the BOU sequence is a three-codon deletion within CDR1 involving codons +28 to +30. In protein RAC, unique substitutions included Thr+5→Val, Pro+7→Leu, Thr/Ser+27→Gly, Ser+29→Thr, Val+33→Leu, Ile+48→Leu, Thr+70→Ser, and Ala+84→Gly. Rare substitutions included Gly+28→Thr, Asn+31→ Lys, and Lys+42→Ile. Two other rare substitutions were common with BOU, Val+96→Trp at the VJ junction and Lys103→Arg within Jλ2. A dozen monoclonal LCs involved in LCDDs, all of the κ type and with an overrepresentation of the Vκ4 subgroup, have been sequenced to date.4Bellotti V Stoppini M Merlini G Zapponi MC Meloni ML Banfi G Ferri G Amino acid sequence of κ Sci, the Bence Jones protein isolated from a patient with light chain deposition disease.Biochim Biophys Acta. 1991; 1097: 177-182Crossref PubMed Scopus (30) Google Scholar, 5Cogné M Preud'homme JL Bauwens M Touchard G Aucouturier P Structure of a monoclonal κ chain of the VκIV subgroup in the kidney and plasma cells in light chain deposition disease.J Clin Invest. 1991; 87: 2186-2190Crossref PubMed Scopus (75) Google Scholar, 7Khamlichi AA Aucouturier P Silvain C Bauwens M Touchard G Preud'homme JL Nau F Cogné M Primary structure of a monoclonal κ chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1992; 87: 122-126Crossref PubMed Scopus (42) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 9Preud'homme JL Aucouturier P Touchard G Khamlichi AA Rocca A Denoroy L Cogné M Monoclonal immunoglobulin deposition disease: a review of immunoglobulin chain alterations.Int J Immunopharmacol. 1994; 16: 425-431Crossref PubMed Scopus (23) Google Scholar, 10Denoroy L Déret S Aucouturier P Overrepresentation of the VκIV subgroup in light chain deposition disease.Immunol Lett. 1994; 42: 63-66Crossref PubMed Scopus (71) Google Scholar, 11Decourt C Cogné M Rocca A Structural peculiarities of a truncated VκIII immunoglobulin light chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1996; 106: 357-361Crossref PubMed Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar We herein describe two λ chains forming amorphous deposits in patients' kidneys. The BOU andRAC LCs were responsible for nonamyloid LC deposits stacked to tubular membrane basements; both cases lacked the prominent glomerulosclerosis that often features Randall-type κ nonamyloid LCDD. Indeed, it has been previously noticed that morphological changes were often less severe and nodular sclerosis was less frequent in λ LCDD than in κ LCDD (13% versus 49% among LCDD cases reported in the literature).12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar Deposits evidenced only by immunofluorescence, without gross morphological alterations of the kidney structures, have also been reported in an experimental model of κ LCDD that represented an initial step of the disease.24Khamlichi AA Rocca A Touchard G Aucouturier P Preud'homme JL Cogné M Role of light chain variable region in myeloma with light chain deposition disease: evidence from an experimental model.Blood. 1995; 86: 3655-3659PubMed Google Scholar The constellation of LCDD and myeloma casts that we report in patient BOU also appear to be unusual and was only present in 2 of 24 patients with LCDD in the study of Strøm et al.12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar Strikingly, both chains are related to the same Vλ2 subgroup25Williams SC Winter G Cloning and sequencing of human immunoglobulin Vλ gene segments.Eur J Immunol. 1993; 23: 1456-1461Crossref PubMed Scopus (143) Google Scholar and encoded by a Vλ segment normally rearranged to Jλ2 and spliced to Cλ2.26Vasicek TJ Leder P Structure and expression of the human immunoglobulin lambda genes.J Exp Med. 1990; 172: 609-620Crossref PubMed Scopus (127) Google Scholar However, given their numerous differences, BOU and RACnucleotide sequences likely derived from two different members of the Vλ2 gene subgroup: BOU is mostly related to the Vλ gene V1-7 (90.8% identity),27Kawasaki K Minoshima S Nakato E Shibuya K Shintani A Schmeits JL Wang J Shimizu N One-megabase sequence analysis of the human immunoglobulin lambda gene locus.Genome Res. 1997; 7: 250-261Crossref PubMed Scopus (175) Google Scholar whereas RAC is mostly related to DPL12 (90.5% identity).25Williams SC Winter G Cloning and sequencing of human immunoglobulin Vλ gene segments.Eur J Immunol. 1993; 23: 1456-1461Crossref PubMed Scopus (143) Google Scholar None of them encodes any potentialN-glycosylation site, but they display a number of features unique among Vλ2 chains: RAC and BOU share a few amino acid substitutions, and both display several replacements introducing hydrophobic residues. The BOU sequence harbors several unusual features within the variable region, both in framework (FR) and in complementary determining regions (CDRs). A striking feature of BOU is a three-residue deletion within the CDR1 between the +28 and +30 positions (according to the numbering of Kabat et al28Kabat EA Wu TT Reid-Miller M Perry HM Gottesman KS Human lambda light chains subgroups 2 and 3. Sequences of Proteins of Immunological Interest. Public Health Service, NIH, Bethesda: US Department of Health and Human Services1991: 118-123Google Scholar), which had never been previously found in any λ2 chain. This three-codon deletion shortens the L1 binding loop and may change its conformation, which is normally helical in λ chains.29Chothia C Lesk AM Canonical structures for the hypervariable regions of immunoglobulins.J Mol Biol. 1987; 196: 901-917Crossref PubMed Scopus (1191) Google Scholar Apart from the CDR1, important changes were also noticed in the CDR3 region, with four unique and two rare amino acid substitutions. In particular, Ser+90→Leu, Ala+92→Val, Ser/Asn+95→Arg, and Thr+95a→Leu may disturb the CDR3 structure by strongly increasing the hydrophobicity of the L3 binding loop.29Chothia C Lesk AM Canonical structures for the hypervariable regions of immunoglobulins.J Mol Biol. 1987; 196: 901-917Crossref PubMed Scopus (1191) Google Scholar As for the FR regions, unique or rare substitutions altogether increasing hydrophobicity include: Ser+2→Ala in the FR1, Ala+43→Val in the FR2, and Ser+65→Phe and Thr+70→Ala in the FR3. The Leu+46→Ile and Ile+48→Leu unique substitutions probably have a limited effect on the protein structure. However, it is noticeable that the Ile+48→Leu substitution is common to BOU and RAC and affects an invariant Ile supposedly implicated in the maintenance of the L2 loop conformation.29Chothia C Lesk AM Canonical structures for the hypervariable regions of immunoglobulins.J Mol Biol. 1987; 196: 901-917Crossref PubMed Scopus (1191) Google Scholar The presence in both proteins of an Asn+60 residue, germinally encoded in BOU and resulting from a substitution in RAC, may also be destabilizing: most LCs carry a negatively charged residue at this position, in the vicinity of a critical Arg+61 to Asp+82 salt bridge usually stabilizing V domains.30Stevens FJ Schiffer M Structure and properties of human immunoglobulin light-chain dimers.Methods Mol Biol. 1995; 51: 51-81PubMed Google Scholar Two other unusual features common toBOU and RAC are the presence of a Trp+96 residue at the end of the CDR3 encoded at the VJ junction and a Lys+103→Arg substitution in the FR4; strikingly, a solvent-exposed Trp features all κ LCDD proteins sequenced to date. All of the other unusual features of protein RAC differ from those of BOU. Although the CDR2 and CDR3 were almost completely canonical, the CDR1 presents three unique substitutions: Ser/Thr+27→Gly; Gly/Ser+29→Thr; and Val+33→Leu and two rare residues, Thr+28 and Lys+31. Hydrophobic amino acids appear in the FR1, Thr+5→Val and Pro+7→Leu, the latter affecting an invariant Pro residue and likely destabilizing the FR1 conformation. Finally, theRAC chain presents an additional Lys+42→Ile substitution in the FR2 and two substitutions within the FR3: Thr+70→Ser and Ala+84→Gly. The herein reported BOU and RAC λ chain sequences are the first to be documented in Randall-type LCDD, in which monoclonal κ chains strongly predominate. The presence of V region peculiarities in LC BOU and RAC was expected from previous sequence analysis of LCDD κ chains4Bellotti V Stoppini M Merlini G Zapponi MC Meloni ML Banfi G Ferri G Amino acid sequence of κ Sci, the Bence Jones protein isolated from a patient with light chain deposition disease.Biochim Biophys Acta. 1991; 1097: 177-182Crossref PubMed Scopus (30) Google Scholar, 5Cogné M Preud'homme JL Bauwens M Touchard G Aucouturier P Structure of a monoclonal κ chain of the VκIV subgroup in the kidney and plasma cells in light chain deposition disease.J Clin Invest. 1991; 87: 2186-2190Crossref PubMed Scopus (75) Google Scholar, 7Khamlichi AA Aucouturier P Silvain C Bauwens M Touchard G Preud'homme JL Nau F Cogné M Primary structure of a monoclonal κ chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1992; 87: 122-126Crossref PubMed Scopus (42) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 11Decourt C Cogné M Rocca A Structural peculiarities of a truncated VκIII immunoglobulin light chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1996; 106: 357-361Crossref PubMed Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar and from direct evidence for the involvement of V region abnormalities obtained in a murine model of human κ LCDD.24Khamlichi AA Rocca A Touchard G Aucouturier P Preud'homme JL Cogné M Role of light chain variable region in myeloma with light chain deposition disease: evidence from an experimental model.Blood. 1995; 86: 3655-3659PubMed Google Scholar It is striking that the herein reported λ chains are closely related. By analogy to the strong implication of λ6 chains in AL-amyloidosis, it may be tempting to speculate that germinally encoded residues of some Vλ2 domains may promote LC aggregation and deposition. However, it is known that the Vλ2 subgroup is overexpressed in myeloma and Waldenström macroglobulinemia (28% of monoclonal Igλ, instead of 3% of Igλ from normal sera),31Solomon A Weiss DT Serologically defined V region subgroups of human λ light chains.J Immunol. 1987; 139: 824-830PubMed Google Scholar, 32Ozaki S Abe M Wolfenbarger D Weiss DT Solomon A Preferential expression of human λ-light chain variable region subgroups in multiple myeloma, AL amyloidosis and Waldenström macroglobulinemia.Clin Immunol Immunopathol. 1994; 71: 183-189Crossref PubMed Scopus (62) Google Scholar and it is clear that not all λ2 chains are responsible for LCDD. In addition, a dozen AL-amyloidosis cases implicating Vλ2 subgroup LC have been reported.31Solomon A Weiss DT Serologically defined V region subgroups of human λ light chains.J Immunol. 1987; 139: 824-830PubMed Google Scholar, 33Sletten K Natvig JB Husby G Juul J The complete primary structure of a prototype immunoglobulin-λ light-chain amyloid fibril protein AR.Biochem J. 1981; 195: 561-572PubMed Google Scholar, 34Picken MM Gallo G Buxbaum J Frangione B Characterization of renal amyloid derived from the variable region of the lambda light chain subgroup II.Am J Pathol. 1986; 124: 82-87PubMed Google Scholar, 35Tveretaas T Sletten K Westermark P The amino acid sequence of a carbohydrate-containing immunoglobulin-light-chain-type amyloid-fibril protein.Biochem J. 1985; 232: 183-190PubMed Google Scholar A likely hypothesis is thus that the λ2 germinally encoded sequences may somehow favor LC aggregation (and in some instances lead to amyloidosis) but that a definitive role in the process of tissue deposition in patients BOU andRAC is played by specific amino acid replacements resulting from somatic mutations and facilitating hydrophobic interactions between LC monomers or dimers. Such replacements would further promote the destabilization and deposition of LC. It is indeed striking thatBOU and RAC λ chains carry a number of unusual replacements, several of them introducing hydrophobic residues. Although crystallization of the proteins will be needed for a definitive assignment of substitutions to solvent-exposed portions of the molecules, several such hydrophobic residues located in the amino-terminal part of the molecule (Ala+2 in BOU and Val+5 and Leu+7 in RAC) or in CDR regions (Val+51, Leu+90, Val+92, and Leu+95A in BOU, and Leu+33 in RAC) are likely to altogether increase hydrophobicity at the surface of both LCs and may play a destabilizing role. Hydrophobic residues may participate in interchain hydrophobic interactions leading to aggregation and thus promote tissue deposition. Similarly, substitutions introducing hydrophobic residues in solvent-exposed portions of LCs have been previously pointed out for several κ LCs implicated in LCDDs4Bellotti V Stoppini M Merlini G Zapponi MC Meloni ML Banfi G Ferri G Amino acid sequence of κ Sci, the Bence Jones protein isolated from a patient with light chain deposition disease.Biochim Biophys Acta. 1991; 1097: 177-182Crossref PubMed Scopus (30) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 11Decourt C Cogné M Rocca A Structural peculiarities of a truncated VκIII immunoglobulin light chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1996; 106: 357-361Crossref PubMed Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar as well as for LCs involved in amyloid fibril formation.15Aucouturier P Khamlichi AA Preud'homme J Bauwens M Touchard G Cogné M Complementary DNA sequence of human amyloidogenic immunoglobulin light chain precursors.Biochem J. 1992; 285: 149-152Crossref PubMed Scopus (28) Google Scholar, 16Hurle MR Helms LR Li L Chan W Wetzel R A role for destabilizing amino acid replacements in light chain amyloidosis.Proc Natl Acad Sci USA. 1994; 91: 5446-5450Crossref PubMed Scopus (329) Google Scholar, 17Stevens PW Raffen R Hanson DK Deng YL Berrios-Hammond M Westholm FA Murphy C Eulitz M Wetzel R Solomon A Schiffer M Stevens F Recombinant immunoglobulin variable domains generated from synthetic genes provide a system for in vitro characterization of light-chain amyloid proteins.Protein Sci. 1995; 4: 421-432Crossref PubMed Scopus (107) Google Scholar These new sequences extend the short list of characterized LCs involved in LCDDs cases and will hopefully help to understand the process by which LCs of decreased solubility or stability can interact, aggregate in high-order polymers, and form deposits in tissues. It also appears likely that structural properties of a given LC are directly correlated to the extent of visceral deposition occurring in the patient and to the prognosis. In that sense, the herein reported λ LCDD cases with high-level secretion of the LC and minimal pathological alterations strikingly contrast with many reported κ LCDD cases in which low or even undetectable secretion of the LC is associated with extensive visceral deposition and renal morphological alterations.5Cogné M Preud'homme JL Bauwens M Touchard G Aucouturier P Structure of a monoclonal κ chain of the VκIV subgroup in the kidney and plasma cells in light chain deposition disease.J Clin Invest. 1991; 87: 2186-2190Crossref PubMed Scopus (75) Google Scholar, 7Khamlichi AA Aucouturier P Silvain C Bauwens M Touchard G Preud'homme JL Nau F Cogné M Primary structure of a monoclonal κ chain in myeloma with light chain deposition disease.Clin Exp Immunol. 1992; 87: 122-126Crossref PubMed Scopus (42) Google Scholar, 8Rocca A Khamlichi AA Aucouturier P Noël LH Denoroy L Preud'homme JL Cogné M Primary structure of a variable region of the VκI subgroup (ISE) in light chain deposition disease.Clin Exp Immunol. 1993; 91: 506-509Crossref PubMed Scopus (49) Google Scholar, 9Preud'homme JL Aucouturier P Touchard G Khamlichi AA Rocca A Denoroy L Cogné M Monoclonal immunoglobulin deposition disease: a review of immunoglobulin chain alterations.Int J Immunopharmacol. 1994; 16: 425-431Crossref PubMed Scopus (23) Google Scholar, 12Strøm EH Fogazzi GB Banfi G Pozzi C Mihatsch MJ Light chain deposition disease of the kidney: morphological aspects in 24 patients.Virchows Arch. 1994; 425: 271-280Crossref PubMed Scopus (57) Google Scholar, 13Gallo G Goni F Boctor F Vidal R Kumar A Stevens FJ Frangione B Ghiso J Light chain cardiomyopathy: structural analysis of the light chain tissue deposits.Am J Pathol. 1996; 148: 1397-1406PubMed Google Scholar, 14Bellotti V Stoppini M Magione PM Fornasieri A Min L Merlini G Ferri G Structural and functional characterization of three human immunoglobulin k light chains with different pathological implications.Biochim Biophys Acta. 1996; 1317: 161-167Crossref PubMed Scopus (25) Google Scholar We thank Dr F. Stevens for helpful comments on λ LC sequences.
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