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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

Here, we present a protocol for direct, early stage guanidinylation that enables rapid total synthesis of aminoguanidine-containing small organic molecules. An advanced synthetic intermediate used in the synthesis of a blood coagulation factor XIa inhibitor was prepared using this protocol.

Abstract

The guanidine functional group, displayed most prominently in the amino acid arginine, one of the fundamental building blocks of life, is an important structural element found in many complex natural products and pharmaceuticals. Owing to the continual discovery of new guanidine-containing natural products and designed small molecules, rapid and efficient guanidinylation methods are of keen interest to synthetic and medicinal organic chemists. Because the nucleophilicity and basicity of guanidines can affect subsequent chemical transformations, traditional, indirect guanidinylation is typically pursued. Indirect methods commonly employ multiple protection steps involving a latent amine precursor, such as an azide, phthalimide, or carbamate. By circumventing these circuitous methods and employing a direct guanidinylation reaction early in the synthetic sequence, it was possible to forge the linear terminal guanidine containing backbone of clavatadine A to realize a short and streamlined synthesis of this potent factor XIa inhibitor. In practice, guanidine hydrochloride is elaborated with a carefully constructed protecting array that is optimized to survive the synthetic steps to come. In the preparation of clavatadine A, direct guanidinylation of a commercially available diamine eliminated two unnecessary steps from its synthesis. Coupled with the wide variety of known guanidine protecting groups, direct guanidinylation evinces a succinct and efficient practicality inherent to methods that find a home in a synthetic chemist's toolbox.

Introduction

The objective of this video is to show how using a direct and early guanidinylation method to make a terminal guanidine structure is more practical, rapid, and efficient than traditional guanidinylation methods in organic synthesis. The guanidine functional group, found on the amino acid arginine, is a key structural element in many complex natural products and pharmaceuticals. The discovery and design of new guanidine containing natural products and small molecules establish the need for a more efficient guanidinylation method. The commonly used circuitous approach features the introduction of a latent guanidine precursor that is unmasked at a late stage in the synthesis. In contrast, a straightforward tactic installs a protected guanidine onto a primary amine early in a synthetic route.

The reactive nature of guanidines generally precludes them from routine use without an appropriate protecting group strategy. Traditionally, methods to add a guanidine functional group involved an indirect approach that involved multiple protection steps followed by adding the guanidine at the end of the synthesis. Two recent syntheses illustrate the drawbacks inherent to indirect guanidinylation1,2. The direct method reported herein involves reacting a protected guanidine reagent with a primary amine early on in the synthesis of a given molecule and then deprotecting it at the end of the synthesis. This strategy was deployed successfully in recent total synthesis of biologically active marine alkaloids clavatadine A and phidianidine A and B3,4.

While this direct guanidinylation method does have its advantages over traditional methods of guanidinylation it still has its drawbacks. The chemical conditions that the protected guanidine can survive will depend on the protecting group employed. Despite these potential drawbacks, the direct guanidinylation method is an enabling strategy to add terminal guanidines to primary amines for use in the synthesis of complex organic molecules.

Protocol

Caution: Please consult and heed Safety Data Sheets (SDS) for each chemical prior to use. A few of the chemicals used in this synthesis are corrosive, toxic, carcinogenic, or otherwise harmful. Consequently, take every precaution to avoid inhalation, ingestion, or skin contact with these chemicals. Please wear appropriate Personal Protective Equipment (PPE) correctly. Proper PPE includes wrap-around safety goggles, nitrile gloves or more chemically resistant gloves, a lab coat, long pants that cover the tops of the shoes, closed-toe shoes. Use a working fume hood with the sash at the lowest possible height, in tandem with additional relevant engineering controls, to minimize the risk of accidental exposure. Portions of the procedure involve standard air- and moisture-free technique, such as the use of a Schlenk line, amber chemical storage bottles with crown caps and elastomer discs, syringe and cannula transfer of liquids and solutions, compressed gasses, and the distillation of flammable liquids under inert atmosphere.5

1. Direct Guanidinylation

  1. Direct guanidinylation of butane-1,4-diamine (5) with Goodman's reagent (6) to prepare di-tert-butoxycarbonyl (Boc)-agmatine (7)3,6
    1. Dry a 1,000 ml, three-necked, round-bottomed reaction flask containing a magnetic stir bar, a 50 ml pressure-equalizing addition funnel, and a 14/20 to 24/40 ground-glass adapter overnight in a drying oven at or above 130 °C. Remove the flask from the oven and quickly cover the aperture of the right and left necks with rubber septa. Fold the rubber septum over the lip of the flask. To the center neck, affix the glass adapter, followed by the addition funnel.
      NOTE: In lieu of overnight oven drying, the flask and stir bar may be covered with a septum, placed on a Schlenk line under vacuum or inert gas, and flame-dried using a propane torch. Please consult these resources for more detailed information on using septa, a Schlenk line, and an addition funnel.7-9
      1. Cover the top of the addition funnel with a rubber septum, folding the rubber septum over the lip of the flask. Cool the assembled apparatus to room temperature under a positive stream of inert gas using a Schlenk line.
    2. Place the stock bottle of butane-1,4-diamine (5) (melting point 25-28 °C) in a hot-water bath to partially melt the solid chemical. Once a small volume of liquefied butane-1,4-diamine (5) is available, use an oven-warmed Pasteur pipet to transfer 2.32 ml (2.03 g, 0.0231 mol, 3.00 molar equivalents) of compound 5 from the stock bottle to an oven-warmed 10 ml graduated cylinder. Transfer the liquefied diamine 5 to the round-bottomed reaction flask using the Pasteur pipet.
      NOTE: Please consult these resources for more detailed information on using a Pasteur pipet.7,10
    3. Add 320 ml of dichloromethane (CH2Cl2) to the round-bottomed reaction flask from a graduated cylinder at ambient temperature (20 °C). Stir the solution while adding 1.1 ml of triethylamine (Et3N) (0.78 g, 0.0077 mol, 1.00 molar equivalents) from a 2 ml glass plunger syringe fitted with a 12-inch, 20-gauge metal needle with a beveled tip.
      NOTE: Please consult these resources for more detailed information on using a syringe.7,8,10 Also consult this resource (pp. 26-29) for detailed information on using a magnetic stir plate.8
    4. Using an analytical balance, weigh 3.01 g (0.00769 mol, 1.00 molar equivalents) of N,-di-Boc--triflylguanidine (6) (Goodman's reagent).11,12 Pour this solid into a beaker. Dissolve this compound in 25 ml of anhydrous CH2Cl2. Draw this solution into a 50 ml glass plunger syringe fitted with a 12-inch, 20-gauge metal needle with a beveled tip. Dispense this solution from the syringe into the addition funnel, ensuring that the stopcock at the bottom of the funnel is closed.
      NOTE: Please consult these resources for detailed information on using an analytical balance.7,13
    5. While continuing the magnetic stirring on the magnetic stir plate, open the stopcock slowly to allow the solution prepared in step 1.1.4 to drip into the round-bottomed reaction flask at a rate of about one drop every four seconds so that the entire solution is added over approximately 1 hr. When the addition is complete, stir the solution at ambient temperature for 12 hr. Formation of a precipitate or residue that adheres to the flask wall is typically observed throughout the 12 hr of stirring.
  2. Aqueous workup for the isolation of di-Boc-agmatine (7)
    1. After 12 hr, expose the solution to air by removing the septum. Remove the magnetic stir bar using a stir-bar retriever. Pour the colorless solution from the round-bottomed reaction flask into a separatory funnel.
    2. Wash the organic solution with two successive 50 ml portions of saturated aqueous sodium bicarbonate (NaHCO3). After each wash, drain the lower organic layer into a clean Erlenmeyer flask. Pour the upper aqueous layer into a second Erlenmeyer flask. Add the organic layer back to the separatory funnel.
      NOTE: Please consult these resources for more detailed information on extraction and using a separatory funnel.7-9,14
    3. Wash the organic solution with two successive 50 ml portions of water. After each wash, drain the lower organic layer into a clean Erlenmeyer flask. Pour the upper aqueous layer into a second Erlenmeyer flask. Add the organic layer back to the separatory funnel.
    4. Wash the organic solution with one 50 ml portion of brine. Drain the lower organic layer into a clean Erlenmeyer flask, and dry with anhydrous sodium sulfate (Na2SO4). Gravity filter the solution through a funnel fitted with fluted filter paper (coarse-porosity, fast flow, 20-25 micron particle retention) into a clean, tared round-bottomed flask.
      NOTE: Please consult these resources for more detailed information on drying organic solutions using a drying agent.7-9,14 Please consult these resources for more detailed information on gravity filtration.7-9,15
    5. Evaporate the liquid in the round-bottomed flask using a rotary evaporator with the bath temperature at 40 °C and the rotation set to 120 rpm.
      NOTE: Please consult these resources for more detailed information on using a rotary evaporator.7-9,16
  3. Purification of di-Boc-agmatine (7)3,6
    1. Prepare a column for flash chromatography using an eluent of 5:3:2 ethyl acetate (EtOAc)-methanol-Et3N through a stationary phase of silica gel. Use a glass chromatography column that is 3.8 cm wide by 45 cm tall.
      NOTE: Please consult these resources for more detailed information on purifying organic compounds using column chromatography.7-9,17,18
      1. Add diatomaceous earth to the column to form a base that is approximately 2 cm tall. This filtering agent will prevent any dissolved silica gel from contaminating the column fractions. Add eluent until the column of the eluent-diatomaceous earth suspension reaches approximately 10 cm tall, about 40-50 ml. Mix the eluent and diatomaceous earth by gentle swirling to ensure the suspension is uniform, and then allow the solid to settle.
        NOTE: Please consult this resource for more detailed information on using diatomaceous earth as a filtering aid.8
      2. Wet pack the column by making a slurry consisting of 100 g of silica gel and a sufficient volume of eluent to enable the slurry to be easily stirred using a metal spatula. Pour the slurry into the column through a plastic or glass funnel.
      3. Use air pressure to force the eluent through the column such that the efflux flows as a gentle stream of liquid. The rate of eluent flow should be approximately two-linear inches per minute. Stop the flow of eluent when it reaches the level of the silica gel, ensuring that the silica gel is constantly wet with the eluent.
    2. Dissolve the contents of the flask (4.21 g) in a volume of the eluent that is just sufficient to dissolve the crude product completely, about 15-20 ml. Carefully load the solution onto the silica gel without disturbing the silica gel by transferring the solution from the flask to the column using a Pasteur pipet. Tap the column to ensure the top of the silica gel is flat. Drain the eluent so that it reaches the level of the silica gel. Add a small amount of the eluent and repeat.
      NOTE: Please consult this resource for detailed information on dissolving solids using solvents.9
      1. To avoid disturbing the silica gel during the elution of the column, add sand to the top of the silica gel to form a cylinder that is approximately 0.5 to 1 cm in height. Add a few milliliters of eluent to wet the sand. Drain the eluent so that it reaches the level of the sand.
      2. Fill the column with eluent. Use air pressure to force the eluent through the silica gel as described in step 1.3.1.3. Collect the eluent in test tubes, each test tube constituting a fraction of the eluent mixture.
    3. Collect fractions until the product has completely eluted from the column. To determine when this has occurred, spot one out of every few column fractions on a thin-layer chromatography (TLC) plate. Di-Boc agmatine (7) has an Rf of 0.39 in 5:3:2 EtOAc-methanol-Et3N.
      NOTE: Please consult these resources for more detailed information on TLC. 7-9,19,20
    4. Collect all fractions containing the desired product in a tared, round-bottomed flask and evaporate the solvent using a rotary evaporator. Dry the resulting cloudy, pale yellow liquid under high vacuum overnight to remove residual solvent. Dissolve an analytical sample (approximately 5 mg) of the purified product, compound 7 (2.49 g, 98% yield), with 0.75 ml of deuterochloroform (CDCl3) and analyze it by proton (1H) and carbon (13C NMR) spectroscopy.
      NOTE: Please consult these resources for more detailed information on preparing a sample for NMR analysis and conducting an NMR experiment.7-9,21
  4. Synthesis of di-Boc-agmatine isocyanate (8)3
    1. Prepare a clean 100 ml round-bottomed reaction flask containing a magnetic stir bar.
    2. On an analytical balance, add the di-Boc agmatine (7) to the round-bottomed reaction flask using a metal spatula until the added net weight of compound 7 is 1.00 g (0.00303 mol, 1.00 molar equivalents). Add 25 ml of CH2Cl2 to the round-bottomed reaction flask from a graduated cylinder at ambient temperature (20 °C). Place the solution in a water-ice bath to cool the solution to 0 °C.
    3. In a fume hood, use an analytical balance to weigh 0.297 g (0.00303 mol, 1.00 molar equivalents) of triphosgene. Add this solid to the round-bottomed reaction flask by pouring it through a glass or plastic funnel.
      CAUTION: Triphosgene is extremely toxic. Wear two pairs of nitrile gloves when handling this compound. Its vapors are also harmful; therefore, it should only be handled in a working fume hood. Transfer an analytical balance into a working fume hood before weighing triphosgene for this reaction.
    4. While continuing the magnetic stirring, add 25 ml of saturated aqueous NaHCO3 by pouring it into the round-bottomed reaction flask through a glass or plastic funnel. When the addition is complete, vigorously stir the biphasic mixture at 0 °C for 30 min using a magnetic stir plate.
  5. Aqueous workup of di-Boc-agmatine isocyanate (8)3
    1. After 30 min, cease stirring and remove the magnetic stir bar using a stir-bar retriever. Pour the mixture from the round-bottomed reaction flask into a separatory funnel that contains 100 ml of CH2Cl2 and 100 ml of water.
    2. Shake the separatory funnel vigorously to mix the layers. Drain the lower organic portion into a clean Erlenmeyer flask. Extract the aqueous layer with three successive 15 ml portions of CH2Cl2. After each extraction, drain the lower organic layer into the Erlenmeyer flask containing the combined organic extracts. After the three extractions, pour the aqueous layer into a second clean Erlenmeyer flask.
    3. Dry the combined organic extracts with anhydrous Na2SO4. Gravity filter the solution through a funnel fitted with fluted filter paper (coarse-porosity, fast flow, 20-25 micron particle retention) into a clean, tared 250 ml round-bottomed flask.
    4. Evaporate the liquid in the round-bottomed flask using a rotary evaporator with the bath temperature at 40 °C and the rotation set to 120 rpm. Dissolve an analytical sample (approximately 5 mg) of the resulting light brown oil, compound 8 (1.11 g, 103% of theoretical), in CDCl3 and analyze it by 1H and 13C NMR spectroscopy, and infrared (IR) spectroscopy.
      NOTE: The isocyanate degrades within hours at room temperature, and should be used immediately in the next step upon isolation. Please consult these resources for more detailed information on infrared (IR) spectroscopy (reference 7: pp. 269-303; reference 9: pp. 146-147; reference 10: 66-76).7-9

2. Synthesis of Carbamate 9 from di-Boc Agmatine Isocyanate (8) and 2,4-DibromoHGAL (3)3

  1. Set up the reaction of di-Boc agmatine isocyanate (8) with 2,4-dibromoHGAL (3)
    1. Dry a 250 ml round-bottomed reaction flask containing a magnetic stir bar overnight in a drying oven at or above 130 °C. Remove the flask from the oven and quickly cover the flask aperture with a rubber septum. Fold the rubber septum over the lip of the flask. Cool the flask to room temperature under a positive stream of inert gas using a Schlenk line.
      NOTE: In lieu of overnight oven drying, the flask and stir bar may be placed on a Schlenk line under vacuum or inert gas and flame-dried using a propane torch.
    2. Using an analytical balance, weigh 0.933 g (0.00303 mol, 1.00 molar equivalents) of 2,4-dibromoHGAL (3), and add this solid to the round-bottomed reaction flask under a nitrogen umbrella.
      NOTE: 2,4-dibromoHGAL (3) was prepared in two steps from 2,5-(dimethoxyphenyl)acetic acid (1), as shown in Figure 1a.3,22,23 The principal by-product formed during the synthesis of compound 3 is 4-bromoHGAL (4), which is formed after the first bromination of HGAL (2).3 During the purification of compound 3 by column chromatography, continued elution with 1:1 EtOAc-hexane permits collection compound 4, which has an Rf of 0.34 when the TLC eluent is 1:1 EtOAc-hexane.3 Typical isolated yields of by-product 4 range from 11-15%.3
    3. Add 30 ml of anhydrous CH2Cl2 to the round-bottomed reaction flask from a glass plunger syringe fitted with a 12-inch, 20-gauge metal needle with a beveled tip, at ambient temperature (20 °C). Stir to dissolve the solid.
      NOTE: Distill the CH2Cl2 over calcium hydride (CaH2) under nitrogen onto activated 3 Å molecular sieves prior to use.
    4. Add 0.103 ml of Hünig's base (0.0078 g, 0.000606 mol, 0.2 molar equivalents) to the round-bottomed reaction flask by syringe.
      NOTE: "By syringe" means that the liquid was collected and dispensed using a metal/polytetrafluoroethylene-coated plunger, gas-tight syringe (glass barrel) fitted with a 6-inch, 20-gauge metal needle with a beveled tip. Distill the Hünig's base over CaH2 under nitrogen onto activated 3 Å molecular sieves prior to use.
    5. Cover the opening of the round-bottomed flask containing the unpurified isocyanate 8 from step 1.5.4 with a rubber septum. Fold the septum over the lip of the flask. Connect the flask to the Schlenk line and purge the flask with nitrogen gas for 10 minutes.
    6. To the flask containing isocyanate 8, add 30 ml of anhydrous CH2Cl2 from a glass-plunger syringe fitted with a 12-inch, 20-gauge metal needle with a beveled tip at ambient temperature (20 °C). Swirl the flask to dissolve the solid.
  2. Transfer the solution of isocyanate 8 to the 2,4-dibromoHGAL (3) and Hünig's base by cannula
    1. Directly connect the two flasks by puncturing each septum with either beveled metal tip of an 18-inch long, 20-gauge metal cannula.
      NOTE: Please consult this resource for more detailed information on using a cannula to transfer one solution to another under inert atmosphere (reference 8: pp. 74-79).8
    2. Remove the nitrogen inlet from the flask containing the CH2Cl2 solution of 2,4-dibromoHGAL (3) and Hünig's base, and insert a 2.5 cm disposable 16-gauge metal needle (exit needle) through the septum. Close the bubbler that serves as the exit port of the Schlenk line.
      CAUTION: Closing off the bubbler of a Schlenk line that is under positive inert gas pressure can be dangerous. Ensure that the exit needle is unobstructed before closing off the bubbler.
    3. Lower one end of the metal cannula into the CH2Cl2 solution of isocyanate 8, and transfer the entire solution to the round-bottomed reaction flask over approximately 1 hr. Adjust the nitrogen pressure as needed for the desired flow rate of approximately 0.5 ml per minute.
    4. Rinse the flask that contained isocyanate 8 with two successive 5 ml portions of CH2Cl2. Transfer each CH2Cl2 rinse by cannula into the round-bottomed reaction flask.
    5. After transferring both rinses into the reaction flask, disassemble the cannula apparatus.
      1. Remove the exit needle from the reaction flask while simultaneously reopening nitrogen flow to the bubbler. Transfer the nitrogen inlet originating from the Schlenk line from the flask that contained the isocyanate to the round-bottomed reaction flask.
    6. Remove the cannula from the round-bottomed reaction flask, and stir the solution at ambient temperature for 3 hr.
  3. Purification of carbamate 93
    1. After 3 hr, expose the solution to air by removing the septum. Remove the magnetic stir bar using a stir-bar retriever.
    2. Evaporate the liquid in the round-bottomed reaction flask using a rotary evaporator with the bath temperature at 40 °C and the rotation set to 120 rpm.
    3. Purify the crude product by flash column chromatography using a gradient elution of 100:0 to 90:10 CH2Cl2-diethyl ether (Et2O) through a stationary phase of silica gel. Use a glass chromatography column that is 3.8 cm wide by 45 cm tall.
    4. Wet pack the column by making a slurry consisting of 60 g of silica gel and a sufficient volume of CH2Cl2 to enable the slurry to be poured into the column.
    5. Use air pressure to force the eluent through the column such that the efflux flows as a gentle stream of liquid. The rate of eluent flow should be approximately two-linear inches per minute. Stop the flow of eluent when it reaches the level of the silica gel, ensuring that the silica gel is constantly wet with the eluent.
    6. Dissolve the crude product (2.202 g, 110% of theoretical) in a minimum volume of CH2Cl2. Carefully load the solution onto the silica gel without disturbing the silica gel. Tap the column to ensure the top of the silica gel is flat. Drain the eluent so that it reaches the level of the silica gel. Add a small amount of CH2Cl2 and repeat.
    7. To avoid disturbing the silica gel during the elution of the column, add sand to the top of the silica gel to form a cylinder that is approximately 0.5 to 1 cm in height. Add a few milliliters of CH2Cl2 to wet the sand. Drain the eluent so that it reaches the level of the sand.
    8. Fill the column with CH2Cl2. Use air pressure to force the eluent through the silica gel as described in step 2.3.5. Collect the eluent in test tubes, each test tube constituting a fraction of the eluent mixture.
    9. Collect fractions until the first compound has completely eluted from the column. To determine when this has occurred, spot one out of every few column fractions on a TLC plate.
      NOTE: The first compound to elute is unreacted 2,4-dibromoHGAL (3), which has an Rf of 0.74 in 90:10 CH2Cl2-Et2O.
    10. When the unreacted 2,4-dibromoHGAL (3) has eluted from the column, replace the eluent with 90:10 CH2Cl2-Et2O. Continue to collect fractions until the desired product has completely eluted from the column. To determine when this has occurred, spot one out of every few column fractions on a TLC plate.
      NOTE: The desired product, carbamate 9, has an Rf of 0.31 in 90:10 CH2Cl2-Et2O.
    11. Collect all fractions containing the carbamate 9 in a tared, round-bottomed flask and evaporate the solvent using a rotary evaporator. Dry the resulting foamy solid to dryness under high vacuum. Analyze an analytical sample (approximately 5 mg) of the product, carbamate 9 (1.36 g, 68% yield), by 1H and 13C NMR in CDCl3. Also collect 1H and 13C NMR spectra in deuterated dimethylsulfoxide (DMSO-d6), which permits direct solvent comparison with the product of step 3.

3. Synthesis and Isolation of Clavatadine A (10)3

  1. Prepare clavatadine A (10) by concomitant acid-catalyzed lactone hydrolysis and guanidine deprotection of carbamate 9
    1. Prepare a clean 250 ml round-bottomed reaction flask containing a magnetic stir bar.
    2. On an analytical balance, weigh 1.205 g (0.00181 mol, 1.00 molar equivalents) of carbamate 9, prepared in step 2, and add this solid to the round-bottomed reaction flask.
    3. Add 12 ml of tetrahydrofuran (THF) to the round-bottomed reaction flask from a graduated cylinder at ambient temperature (20 °C). The solid should dissolve as the solution is stirred.
    4. Prepare 48 ml of 1.0 M aqueous hydrochloric acid (HCl).
      1. Add 4 ml of concentrated (12.0 M) HCl solution to a 10 ml graduated cylinder.
      2. Transfer the concentrated HCl solution by Pasteur pipet to a 50 ml graduated cylinder that contains 30-40 ml of distilled water. Dilute this solution with distilled water to a final volume of 48 ml.
    5. Add the 48 ml of aqueous 1.0 M HCl solution prepared in step 3.1.4.3 to the round-bottomed reaction flask at ambient temperature with stirring.
    6. Gently place a 24/40 ground-glass stopper to cover the aperture of the reaction flask.
    7. Submerse the reaction flask in a water bath that has been preheated to 30 °C on a temperature-controlled hot plate. Ensure that the level of the solution in the reaction flask is below the water level in the bath.
      NOTE: At this scale, the reaction will produce 2 molar equivalents of carbon dioxide and 2 molar equivalents of isobutene gas, which should occupy a space of approximately 0.174 L. Ensure the stopper is placed lightly on the flask to ensure that any excess pressure that develops can be released through the ground-glass joint.
    8. While continuing the magnetic stirring, heat the solution at 30 °C for 20 hr.
    9. After 20 hr, vacuum filter the resulting suspension through a medium porosity sintered-glass funnel into a clean, tared round-bottomed flask to remove any insoluble material.
    10. Evaporate the yellow-colored solution in the reaction flask using a rotary evaporator with the bath temperature at 50 °C and the rotation set to 120 rpm.
    11. Dry the resulting yellow- to peach-colored amorphous solid to constant weight under high vacuum. Facilitate drying by heating the evacuated flask in a warm (40 °C) water bath.
    12. Dissolve an analytical sample (approximately 5 mg) of the product, which is the hydrochloride salt of clavatadine A (10) (0.866 g, 93% yield), in anhydrous DMSO-d6, and analyze it by one-dimensional 1H and 13C NMR spectroscopy.

Results

Direct guanidinylation of a commercially available α,ω-diamine, followed by reaction with triphosgene, afforded the reactive isocyanate 8 as the linear portion of clavatadine A (Figure 1b). Yields of this two-step reaction sequence are invariably high, 95% or greater. Guanidinylation reagent 6 was prepared exactly as described by Goodman.11,24

When isocyanat...

Discussion

Initial efforts to prepare clavatadine A enlisted a traditional, indirect approach to guanidinylation from a suitable amine precursor, which in this case was a terminal azide. Central to this effort was the union of the two halves of the molecule to construct the carbamate moiety. Unfortunately, all attempts to realize an azide reduction in anticipation of a planned late-stage guanidinylation were unsuccessful.25,26 These setbacks inspired the pursuit of compound 7, which could be prepared in ...

Disclosures

The authors have nothing to declare.

Acknowledgements

We thank Dr. John Greaves and Ms. Soroosh Sorooshian, Department of Chemistry, University of California, Irvine Mass Spectrometry Facility, for mass spectrometric analyses. We also thank Mr. Jacob Buchanan for helpful discussions, as well as Miss Stephanie J. Conn, Mrs. Shannon M. Huffman (Vreeland), and Miss Alexandra N. Wexler for early stage work on this project. Partial funding was provided by the Central Washington University (CWU) School of Graduate Studies (C.E.M), the CWU Seed Grant Program, and the CWU Faculty Research Program.

Materials

NameCompanyCatalog NumberComments
Chloroform-dSigma-Aldrich612200-100G99.8% D, 0.05% v/v tetramethylsilane; Caution: toxic
Dimethylsulfoxide-d6185965-50G99.9% D, 1% v/v tetramethylsilane
sodium thiosulfate pentahydrateSigma-AldrichS8503-2.5KG
sodium sulfate, anhydrousSigma-Aldrich238597-2.5KG
silica gelFisher ScientificS825-25Merck, Grade 60, 230-400 mesh
washed sea sandSigma-Aldrich274739-5KG
hexaneSigma-Aldrich178918-20LCaution: flammable
ethyl acetateSigma-Aldrich319902-4L
methylene chlorideSigma-AldrichD65100-4L
sodium chlorideSigma-AldrichS9888-10KG
sodium bicarbonateSigma-AldrichS6014-2.5KG
acetic acidSigma-Aldrich695092-2.5L
hydrochloric acidSigma-Aldrich258248-2.5LCaution: Corrosive
bromineSigma-Aldrich470864-50G>99.99% trace metals basis; Caution: Corrosive, causes severe burns
hydrobromic acidSigma-Aldrich244260-500ML48% aqueous; Caution: Corrosive
2,5-dimethoxyphenylacetic acidChemImpex26909
chloroformSigma-Aldrich132950-4LCaution: Toxic
tetrahydrofuranSigma-Aldrich360589-4x4LCaution: highly flammable
N,N-diisopropylethylamineSigma-AldrichD125806-500MLCaution: Corrosive
triethylamineSigma-AldrichT0886-1LCaution: Corrosive
3 Angstrom molecular sievesSigma-Aldrich208574-1KG
calcium hydrideSigma-Aldrich213268-100GCaution: Corrosive, reacts violently with water
ammonium molybdateSigma-Aldrich431346-50G
phosphomolybdic acidSigma-Aldrich221856-100G
cerium(IV) sulfateSigma-Aldrich359009-25G
1-butanolSigma-Aldrich537993-1L
1,4-butanediamineSigma-AldrichD13208-100GCaution: Corrosive / warm in hot water bath to melt prior to use
triphosgeneVWR200015-064Caution: Highly Toxic
methanolSigma-Aldrich646377-4X4L
sodium acetateSigma-Aldrich241245-100G
Dimethylsulfoxide-d6Sigma-Aldrich570672-50GAnhydrous, 99.9% D
sodium hydroxideSigma-Aldrich221465-500GCaution: Corrosive
guanidine hydrochlorideSigma-AldrichG4505-25GCaution: Toxic, Corrosive
di-tert-butyl dicarbonateVWR200002-018%Caution: Toxic / may warm in hot water bath to melt prior to use
trifluoromethanesulfonic anhydrideFisher Scientific50-206-77198%, anhydrous; Caution: toxic, corrosive, extremely moisture sensitive

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