Control of potato cyst-nematodes, Heterodera rostochiensis and H. pallida, in sandy, peaty and silt loam soils by oximecarbamate and organophosphate nematicides

Small amounts (5.6 or n-2 kg a.i./ha) of aldicarb or oxamyl, incorporated in the soil before potatoes were planted in spring, controlled potato cyst-nematodes (Heterodera rostochiensis and H. pallida) on susceptible cultivars equally well in sandy, peaty and silt loam soils. In soils treated with either nematicide, nematode numbers increased little or decreased; in untreated soils nematode numbers increased greatly. In contrast organophosphate nematicides, similarly applied, fenamiphos (proposed BSI common name for O-ethyl-O-(3-methyl-4-methylthiophenyI)-isopropylamido-phosphate), ethoprophos (proposed BSI common name for (O-ethyl S, 5-dipropyl phos-phorodithioate), CGA 12223 (O, O-diethyl O-[i-isopropyl-5-chloro-i,2,4-triazoIyl-(3)] phosphorothioate) and Dowco 275 (O, O-diethyl O-(6-fluoro-2 pyridyl) phosphorothioate), were ineffective at one or more of the experimental sites. Potato yields were greatly increased by oximecarbamate or organophosphate nematicides only in soils heavily infested with the nematodes.     

Laboratory and field tests in 1966-67 on chemical control of wireworms (Agriotes spp.)

Of sixteen compounds applied to soil in laboratory tests, azinphos-ethyl, P2188 (O,O-diethyl S-chloromethyl phosphorothiolothionate), ‘Dursban’ (O,O-diethyl O-3,5,6-trichloro-2-pyridyl phosphorothioate), P1973 (S-(N-methoxycarbonyl-N-methylcarbamoylmethyl) dimethyl phosphorothiolothionate), B77488 (O,O-diethylphosphorothioate O-esterwith phenylglyoxylonitrile oxime) and R42211 (O,O-diethyl O-(2-diethylamino-6-methyl-pyrimidin-4-yl) phosphorothioate) killed wireworms when first tested, but in second tests with the same soils only ‘Dursban’, P2188 and B77488 did so. Treating seeds with ‘Dyfonate’ (O-ethyl S-phenyl ethyl phosphonodithioate) or with ethion/γ-BHC mixtures killed few wireworms. Three field trials compared the organophosphorus insecticides ‘Dursban’, ‘Dyfonate’ and phorate with organochlorine standards. In trials with barley and potatoes the standard was 3 lb a.i./acre (3·36 kg/ha) of aldrin. The organophosphorus compounds increased plant stands of barley almost as much as aldrin, although they killed fewer wireworms; and they protected fewer potato tubers from wireworm damage. The third trial compared the organophosphorus compounds with 0·5 lb a.i./acre (0·56 kg/ha) γ-BHC sprayed on a site drilled with sugar beet seed dressed with dieldrin. The γ-BHC increased plant stands almost as much as did 3 lb a.i./acre of the organophosphorus insecticides, and killed as many wireworms.     

Influence of Organic Pesticides on Nematode Populations and Seed Production of Centipede Grass

Applications of ethyl 4-(methylthio)-m-tolyl isopropylphosphoramidate, O,O-diethyl O-((p-(methylsulfinyl)phenyl) phosphorothioate, and O,O-diethyl S-[2-(ethylthio)ethyll phosphorotbioate effectively controlled Trichodorus christiei on centipede grass. Populations of Pratylenchus spp. and Xiphinema americanum were significantly reduced with a mixture of methanesulfonic acid, 2,4-dichlorophenyl ester and 1,2-dibromo-3-chloropropane. Ethyl 4-(methylthio)-m-tolyl isopropylphosphoramidate and O,O-diethyl O-((p-(methylsulfinyl)phenyl phosphorothioate significantly suppressed populations of Pratylenchus spp., and the latter reduced populations of X. arnericanum. Ethyl 4-(methylthio)-m-tolyl isopropylphosphoramidate and O,O-diethyl O-((p-methylsulfinyl) phenyl) phosphorothioate significantly reduced populations of Criconemoides ornatus. Increased seed production was correlated with nematode control.     

Metabolic Behavior of O-Ethyl S,S-Diphenyl Phosphorodithiolate (edifenphos) in Female Goat

The determination of residues in fresh milk and the metabolic fate of edifenphos (O-ethyl S, S-diphenyl phosphorodithiolate), the active ingredient of the fungicide HINOSAN® were conducted in female goats using gas-liquid chromatographic techniques. Edifenphos was rapidly metabolized to form polar products which were excreted in the urine. The major metabolites found in the urine were O-ethyl S-phenyl hydrogen phosphorothiolate and O-conjugates of m- and p-(hydroxyphenyl) methyl sulfone. Several other metabolites; S, S-diphenyl hydrogen phosphorodithiolate, S-phenyl dihydrogen phosphorothiolate, O-ethyl dihydrogen phosphate, O-ethyl S-phenyl hydrogen phosphorodithiolate and methyl phenyl sulfone were also identified. In the feces, blood, some organs and tissues, edifenphos was scarcely detected. Oral administration of edifenphos to goat at the rate of 10 mg/kg resulted the secretion of 0.0008 ppm of edifenphos in milk as the maximum level after 6 hr of the administration.     

Metabolic Fate of O-Ethyl S,S-Diphenyl Phosphorodithiolate (Hinosan®) in Rice Plant

Metabolism and residual fate of O-ethyl S,S-diphenyl phosphorodithiolate (Hinosan®) applied on rice plant was examined by using ³⁵S-labeled or ³²P-labeled compound. Ion exchange chromatography, thin-layer chromatography and gas-liquid chromatography with flame thermionic detector or flame photometric detector were applied for identification of water soluble and toluene soluble metabolites of Hinosan. Degradation of Hinosan at the initial stage of metabolism was mainly the cleavage of P-S linkage, and a large portion of phenyl dihydrogen phosphorothiolate and a minor portion of O-ethyl S-phenyl hydrogen phosphorothiolate were found as water soluble metabolites. Phenylthio radical released on the production of the above mentioned metabolites was recovered as diphenyl disulfide, which was finally converted to sulfuric acid through benzenesulfonic acid. Triphenyl phosphorotrithiolate and O,O-diethyl S-phenyl phosphorothiolate were produced by transesterification between molecules of Hinosan at the initial stage of metabolism. Examination of metabolites in rice grains showed that sulfur and phosphorus atoms in Hinosan were incorporated into neutral or cationic substances probably after several steps of chemical transformation.     

1-(<Emphasis Type="Italic">N</Emphasis>-Trifluoroacetylamino)alkylphosphonic acids: synthesis and properties

Summary. The 1-(N-trifluoroacetylamino)alkylphosphonic acids (TFA-AA^P) – sub-products in the synthesis of O,O-dialkyl 1-(N-trifluoroacetylamino)alkylphosphonates and O,O-diethyl 1-aminoalkylphosphonates, were synthesized in two-stage transformations of 1-aminoalkylphosphonic acids including: trifluoroacetylation of 1-aminoalkylphosphonic acids (AA^P) using a trifluoroacetic anhydride/trifluoroacetic acid reagent (AA^P + TFAA/TFA→2) and subsequent hydrolysis of the intermediary compounds 2 into desired TFA-AA^P (2→TFA-AA^P). These intermediates 2 presented mixtures of the type of mixed anhydrides of TFAA and 1-(N-trifluoroacetylamino)alkylphosphonic, pyrophosphonic and polyphosphonic acids, which underwent rapid and quantitative conversion to corresponding TFA-AA^P during treatment with an excess of water. The title acids were isolated by direct evaporation of the corresponding post-reaction mixtures, and their physicochemical proprieties, including deacylation abilities, were determined. TFA-AA^P compounds can be re-converted into the starting amino acids AA^P under respectively mild conditions (AA^P→TFA-AA^P→AA^P).     

Synthesis and biological evaluation of O-methyl and O-ethyl NSAID hydroxamic acids

This paper reports the synthesis of O-methyl and O-ethyl NSAID hydroxamic acids, their antimicrobial activities, and their ability to inhibit urease and soybean lipoxygenase activities. Ibuprofen and fenoprofen hydroxamic acids with free hydroxy groups present the highest antimicrobial activity, while indomethacin and diclofenac analogs show significantly lower antimicrobial activity. Diclofenac hydroxamic acid 4e exerts the highest anti-urease activity. Indomethacin O-ethyl hydroxamic acid 3h and ibuprofen O-benzyl hydroxamic acid 4b exert significant inhibitory activities on soybean lipoxygenase. Fenoprofen and indomethacin O-ethyl hydroxamic acids 3b and 3h and diclofenac and indomethacin O-benzyl analogs 4g and 4i highly inhibit lipid peroxidation. The highest antioxidant activity was shown by fenoprofen derivative 3b.     

Regioselective monoacylation of 2-O-α-d-glucopyranosyl-l-ascorbic acid by a polymer catalyst in N,N-dimethylformamide

6-O-Dodecanoyl-2-O-α-d-glucopyranosyl-l-ascorbic acid (6-sDode-AA-2G) was synthesized from 2-O-α-d-glucopyranosyl-l-ascorbic acid and lauric anhydride with a polymer catalyst, poly(4-vinylpyridine), in N,N-dimethylformamide without the introduction of protecting groups. The optimum reaction conditions enabled 6-sDode-AA-2G to be synthesized in a yield of 49.7%. The yield and the regioselectivity in this method were far superior to those in our previous method by using an enzyme. The polymer catalyst could be recycled more than five times without any significant activity loss.     

Acyclic-sugar purine nucleosides derived from -glucose: stereochemical correlations in acyclic-sugar derivatives unequally substituted at c-1

Condensation of 2,3,4,5,6-penta-O-acetyl-l-bromo-1-s-methyl-l-thio- -glucito (1) with 6-chloro-9-(chloromercuri)purine gave 49% of crystalline, levorotatory (1s)-2,3,4,5,6-penta-O-acetyl-1-(6-chloropurin-9-yl)-1- -methyl-1-thio- -glucitol (3), together with a smaller proportion of the syrupy, dextrorotatory (1R) isomer. Thiourea converted 3 into its 6-mercaptopurine analog, whose O-deacetylated derivative could be s-methylated to the corresponding -(methylthio)purin-9-yl analog; all compounds in this sequence were crystalline and were the pure (1s) isomers, as were the corresponding 1′-s-ethyl derivatives prepared by a similar route. Crystal-structure analysis of the O-deacetylated derivative of the 1 s-ethyl analog of 3 established the relative stereochemistry of the ethylthio group, permitting assignment of the (1s) absolute stereochemistry to this compound and thus to all compounds in the sequence starting from 1, including the previously described, crystalline, levorotatory 1-(1,6-dihydro-6-thioxopurin-9-yl)-1-s-ethyl-1-thio- -glucitol, whose chirality at C-1 had not hitherto been established. The close similarity of the chiroptical properties of the crystalline 1′-s-methyl derivatives to those of their 1′-s-ethyl counterparts permitted firm attribution of (1s) chirality to the former series also. Conformational studies showed that all of the derivatives have the sugar chain in a non-extended (sickle) conformation.     

Control of potato cyst-nematode, Globodera rostochiensis, and root-knot nematode, Meloidogyne incognita, by organosphosphorus, carbamate, benzimidazole and other compounds

Control of potato cyst-nematode, Globodera rostochiensis, was examined on potato or tomato in pots and on potato in field plots by various chemicals incorporated into the soil at planting. The most effective nematicides were organophosphorus compounds, generally of the type O,O-diethyl O-phosphoro-thioates or O,O-diethyl phosphorodithioates, carbamates and benzimidazoles. In organic soils, the more lipophilic compounds were less effective, presumably because of sorption onto soil organic matter. Foliar sprays of chemicals, including oxamyl which is known to be translocated to roots, gave poor control of G. rostochiensis. The root-knot nematode, Meloidogyne incognita, on tomato, widely used in screening for nematicidal activity, was controlled by aldicarb or phoxim incorporated into the soil at planting, but not by benomyl or thiabendazole, in contrast to the moderate effectiveness of these latter two chemicals against G. rostochiensis.     

Salicylanilide diethyl phosphates as cholinesterases inhibitors

Based on the presence of dialkyl phosphate moiety, we evaluated twenty-seven salicylanilide diethyl phosphates (diethyl [2-(phenylcarbamoyl)phenyl] phosphates) for the inhibition of acetylcholinesterase (AChE) from electric eel (Electrophorus electricus L.) and butyrylcholinesterase (BChE) from equine serum. Ellman’s spectrophotometric method was used. The inhibitory activity (expressed as IC₅₀ values) was compared with that of the established drugs galantamine and rivastigmine. Salicylanilide diethyl phosphates showed significant activity against both cholinesterases with IC₅₀ values from 0.903 to 86.3 μM. IC₅₀s for BChE were comparatively lower than those obtained for AChE. All of the investigated compounds showed higher inhibition of AChE than rivastigmine, and six of them inhibited BChE more effectively than both rivastigmine and galantamine. In general, derivatives of 4-chlorosalicylic acid showed enhanced activity when compared to derivatives of 5-halogenated salicylic acids, especially against BChE. The most effective inhibitor of AChE was O-{5-chloro-2-[(3-bromophenyl)carbamoyl]phenyl} O,O-diethyl phosphate with IC₅₀ of 35.4 μM, which is also one of the most potent inhibitors of BChE. O-{5-Chloro-2-[(3,4-dichlorophenyl)carbamoyl]phenyl} O,O-diethyl phosphate exhibited in vitro the strongest inhibition of BChE (0.90 μM). Salicylanilide diethyl phosphates act as pseudo-irreversible cholinesterases inhibitors.     

Substituent Effect on Photosynthesis of N2-α-Substituted Benzyl-N4-alkyl-2,4-diamino-6-chloro-s-triazines and Their Phytotoxic Property

The influence of substituents on the activities of a series of N²-α-substituted benzyl-N⁴-alkyl-2,4-diamino-6-chloro-s-triazines as inhibitors of photosystem II (PSII) was examined, and the phytotoxic differences between them and atrazine, as to the photosynthesis in leaf disks, mesophyll cells, intact chloroplasts and broken chloroplasts of spinach, and as to seedling-growth, were discussed. The inhibitory activity of the N²-α,α-dimethylbenzyl-N⁴-ethyl derivative (6), which was comparable on that of atrazine, was lower than those of the N²-α-alkylbenzyl analogues (1 ~5). The N⁴-?-alkyl-N²-α- methylbenzyl derivatives, in spite of the carbon length of the alkyl group, exhibited more potent activity than atrazine, but an a α β substitution of the N⁴-n-alkyl group caused a decrease in the activity with a few exceptions. These data may imply that the space of the binding site on PSII surrounding both the N² and N⁴ amino groups is relatively large. The binding between the receptor site and the N⁴ amino group, however, is easily influenced by a slight structural change in an inhibitor. The herbicidal compounds, N²-α-methylbenzyl-A^⁴-ethyl (1), A^²-α,α-dimethylbenzyl-N⁴-1-methylpropyl (30) and N²-α-methylbenzyl-N⁴,N⁴-diethyl (42) derivatives, exhibited potent inhibitory activity in the seedling growth test under dark/light conditions, whereas atrazine was very poor. The inhibitory activity of compound (1) toward photosynthesis was poor with leaf disks, compared to atrazine, whereas, the order of their activities was the reverse for plant preparations such as abaxial epidermis peeled leaf disks, mesophyll cells, intact chloroplasts and broken chloroplasts. It was indicated that a change in the phytotoxic symptom in the whole plant assay would be correlated to the permeability of the compound through the plant membrane(s).     

Effects of insecticide profenophos on germination,early growth,meiotic behavior and chlorophyll mutation of barley (<Emphasis Type="Italic">Hordeum vulgare</Emphasis> L.)

The genotoxicity of different concentrations of insecticide, profenophos (O-4-bromo-2-chlorophenyl O-ethyl S-propyl phosphorothioate) was evaluated at various stages of cell cycle (G₁, S and G₂) by using the seeds of barley (Hordeum vulgare L.). The aim of this work was to investigate the effects of insecticide profenophos at various stages of cell cycle on germination, seedling height and meiotic behavior in M₁ and chlorophyll mutations in M₂ generation. From the present study, it can be concluded that the stages of cell cycle were sensitive for the treatments of chemicals and it also showed that the S-phase of cell cycle is more sensitive than other phases of cell cycle.     

Metabolism of O-Ethyl S,S-Diphenyl Phosphorodithioate (Hinosan®) by Mycelial Cells of Pyricularia oryzae

Metabolism of organophosphorus fungicide Hinosan^® (O-ethyl S, S-diphenyl phosphorodithioate) by mycelia of P. oryzae, rice blast fungus, was studied using ³²P–, ³⁵S– and non-labeled compounds, by ion exchange chromatography, paper chromatography, thin-layer chromatography and gas chromatography, and identifying the metabolites and their derivatives with authentic compounds.

The main metabolic pathway is hydrolysis of one P-S linkage followed by the other P-S linkage or ethyl ester linkage and finally yielding phosphoric acid. A part of the fungicide metabolizes to hydroxylated intermediate metabolite, O-ethyl S-p-hydroxyphenyl S-phenyl phosphorodithioate. No significant difference in rate and mode of metabolism was found in this experiment between susceptible and resistant clones against the fungicide.     

Bacteriochlorophyll c monomers,dimers, and higher aggregates in dichloromethane,chloroform, and carbon tetrachloride

Bacteriochlorophyll c in vivo is a mixture of at least 5 homologs, all of which form aggregates in CH₂Cl₂, CHCl₃ and CCl₄. Three homologs exist mainly in the 2-R-(1-hydroxyethyl) configuration, whereas the other two homologs, 4-isobutyl-5-ethyl and 4-isobutyl-5-methyl farnesyl bacteriochlorophyll c, exist mainly in the 2-S-(1-hydroxyethyl) configuration (Smith KM, Craig GW, Kehres LA and Pfennig N (1983) J. Chromatograph. 281: 209–223). In CCl₄ the S-homologs form an aggregate of 2–3 molecules whose absorption (747 nm maximum) and circular dichroism spectra resemble those of the chlorosome. In CH₂Cl₂, CHCl₃ and CCl₄ the 4-n-propyl homolog (R-configuration) forms dimers absorbing at ca. 680 nm and higher aggregates absorbing at 705–710 nm. In CCl₄ the dimerization constant is approx. 10 µM^–1 (1000 times that for chlorophyll a). The difference between the types of aggregates formed by the 4-n-propyl and 4-isobutyl homologs is attributed to the difference between the R- and S-configurations of the 2-(1-hydroxyethyl) groups in each chlorophyll.Abbreviations BChl bacteriochlorophyll - CD circular dichroism - Chl chlorophyll - DNS data not shown - EEF 4-ethyl-5-ethyl farnesyl - iBM/EF 4-isobutyl-5-methyl/ethyl farnesyl - MEF 4-methyl-5-ethyl farnesyl - PEP 4-n-propyl-5-ethyl farnesyl     

Structural Characterization of Lignin during Pinus taeda Wood Treatment with Ceriporiopsis subvermispora

Pinus taeda wood chips were biotreated with Ceriporiopsis subvermispora under solid-state fermentation for periods varying from 15 to 90 days. Milled wood lignins extracted from sound and biotreated wood samples were characterized by wet-chemical and spectroscopic techniques. Treatment of the lignins by derivatization followed by reductive cleavage (DFRC) made it possible to detect DFRC monomers and dimers that are diagnostic of the occurrence of arylglycerol-β-O-aryl and β-β, β-5, β-1, and 4-O-5 units in the lignin structure. Quantification of these DFRC products indicated that β-O-aryl cleavage was a significant route for lignin biodegradation but that β-β, β-5, β-1, and 4-O-5 linkages were more resistant to the biological attack. The amount of aromatic hydroxyls did not increase with the split of β-O-4 linkages, suggesting that the β-O-4 cleavage products remain as quinone-type structures as detected by UV and visible spectroscopy. Nuclear magnetic resonance techniques also indicated the formation of new substructures containing nonoxygenated, saturated aliphatic carbons (CH₂ and CH₃) in the side chains of lignins extracted from biotreated wood samples.     

Enantiopure O‐Ethyl Phenylphosphonothioic Acid: A Solvating Agent for the Determination of Enantiomeric Excesses

An improved method, which is highly reproducible, was developed for the enantioseparation of racemic O‐ethyl phenylphosphonothioic acid ( 1a ) with brucine by introducing seeding to a supersaturated solution of the diastereomeric salt mixture. The present method gave both diastereomeric salts in high yields with a diastereomeric ratio of >99.5:0.5 upon choosing the crystallization solvent (MeOH for the ( (R)-1a salt and MeOH/H₂O for the ( (S)-1a salt). The enantiopure acid (R)-1a , (S)-1a showed a good chirality recognition ability for not only strong bases, such as amines and amino alcohols, but also weakly basic alcohols and was applicable as a solvating agent to the ¹H NMR determination of the enantiomeric excess of chiral amines, amino alcohols, and alcohols, including aliphatic substrates. Chirality 26:614–619, 2014. © 2014 Wiley Periodicals, Inc.     

Enantiopure cyclic O‐substituted phenylphosphonothioic acid: Synthesis and chirality‐recognition ability

As a new acidic selector (resolving agent), we synthesized an enantiopure O‐alkyl phenylphosphonothioic acid with a seven‐membered ring ((R)‐ 5 ), which was designed on the basis of the results for the enantioseparation of 1‐arylethylamine derivatives with acyclic O‐ethyl phenylphosphonothioic acid ( I ). The phosphonothioic acid (R)‐ 5 showed unique chirality‐recognition ability in the enantioseparation of 1‐naphthylethylamine derivatives, aliphatic secondary amines, and amino alcohols; the ability was complementary to that of I . The X‐ray crystallographic analyses of the less‐ and more‐soluble diastereomeric salts showed that hydrogen‐bonding networks in the salt crystals are 2₁‐column‐type with a single exception which is cluster‐type. In the cases of the 2₁‐column‐type crystals, stability of the crystals is firstly governed by hydrogen bonds to form a 2₁‐column and secondly determined by intra‐columnar T‐shaped CH/π interaction(s), intra‐columnar hydrogen bond(s), inter‐columnar van der Waals interaction and/or inter‐columnar T‐shaped CH/π interaction(s). In contrast, the cluster‐type salt crystal is stabilized by the assistance of inter‐cluster T‐shaped CH/π and van der Waals interactions. To realize still more numbers of intra‐ and inter‐columnar and ‐cluster T‐shaped CH/π interactions, the seven‐membered ring of (R)‐ 5 plays a considerable role. Chirality 23:438–448, 2011. © 2009 Wiley‐Liss, Inc.     

Oxidation of the erythro and threo forms of the phenolic lignin model compound 1-(4-hydroxy-3-methoxyphenyl)-2-(2-methoxyphenoxy)-1,3-propanediol by laccases and model oxidants

Mixtures of equal amounts of the erythro and threo forms of the phenolic arylglycerol β-aryl ether 1-(4-hydroxy-3-methoxyphenyl)-2-(2-methoxyphenoxy)-1,3-propanediol were oxidized (i) with laccases from Trametes versicolor, Agaricus bisporus, Myceliophthora thermophila and Rhus vernicifera, (ii) with laccase-mediator systems consisting of T. versicolor laccase and ABTS or HBT, and (iii) with various model oxidants including cerium(IV) ammonium nitrate (CAN), lignin peroxidase, Fenton’s reagent, and lead(IV) tetraacetate (LTA). All the laccases exhibited a similar preferential degradation of the threo form. The mediator ABTS counteracted the threo preference of laccase, but the mediator HBT did not affect it. The outer-sphere model oxidants CAN and lignin peroxidase showed a preferential degradation of the threo form. LTA and Fenton’s reagent did not exhibit any stereo-preference. The results suggest that laccases of different origin, primary structure, and redox potential behave as typical outer-sphere oxidants in their interaction with the diastereomers of the arylglycerol β-aryl ether.     

Nα-Fmoc-O,O-(dimethylphospho)-L-tyrosine fluoride: A convenient building block for the solid-phase synthesis of phosphotyrosyl peptides

Summary Fmoc-O,O-(dimethylphospho)-l-tyrosine was converted into stable Fmoc-O,O-(dimethylphospho)-L-tyrosine fluoride by means of (diethylamino) sulfur trifluoride or cyanuric fluoride. This building block was used for efficient coupling of phosphotyrosine to the adjacent sterically hindered amino acid Aib or Ac₆c in, model peptide sequences as well as for the synthesis of the ‘difficult’ phosphotyrosine peptide Stat91^695–708. The phosphate methyl groups were cleaved on solid phase after peptide assembly by means of trimethylsilyl iodide in MeCN. Aib, α-aminoisobutyric acid Ac₆c, 1-amino-cyclohexyl-l-carboxylic acid; BOP, benzotriazol-l-yl-oxy-tris(dimethylamino) phosphonium hexafluorophosphate, CIP, 2-chloro-l, 3-dimethylimidazolidium hexafluorophosphate, DAST, (diethylamino)sulfur trifluoride; DBU 1,8-diazabicyclo[5.4.0]undec-7-ene; DCM, dichloromethane; DIEA, drisopropylethylamine; DMA dimethylacetamide; Fmoc, 9-fluorenylmethoxycarbonyl; HATU,O-(7-azabenzotriazol-l-yl)-1.1,3,3-tetramethyluronium hexafluorophosphate; HOAt, I-hydroxy-7-azabenzotriazole; HOBt,N-hydroxybenzotriazole; HPLC, high-performance liquid chromatography; MBHA, 4-methylbenzhydrylamine; MeCN, acetonitrile; NMP,N-methyl-2-pyrrolidinone; NMR, nuerear magnetic resonance; PS, polystyrene; PyBroP, bromotris(pyrrolidino)phosphonium hexafluorophosphate; Rink amide MBHA-PS, 4-(2′,4′-dimethoxyphenyl-Fmoc-aminophenyl)-phenoxyacetamido-norleucyl-MBHA-PS; TFA, trifluoroacetic acid; TMSI, trimethylsilyl iodide; TPTU, 2-(2-pyridon-l-yl)-1,1,3,3-tetramethyluroniumfluoroborate; t_R, retention time; UNCA, arethane-protected amino acidN-carboxy anhydride Abbreviations for amino acids and nomenclature of, peptide structures follow the recommendations of the IUPAC-IUB Commission on Biochemical Nomenclature [Eur. J. Biochem., 138 (1984) 9].