IE75663B1 - Use of chelate complexes - Google Patents

Description

USE OF CHELATE COMPLEXES This application has been divided from our co-pending Irish Patent Application No. 2076/87 dated 31st July 1987 which relates to NNR imaging with paramagnetic polyvalent metal salts of poly-(acidalkylene-amino)-alkanes.

The present invention relates to improvements in the enhancing of nuclear, magnetic resonance (NMR) imaging of animal tissues, especially cardiac and liver.

X-rays have long been used to produce images of 15 animal tissue, e.g. the internal organs of a patient, the patient being positioned between a source of X-rays and a film sensitive to the rays. Where organs interfere with the passage of the rays, the film is less exposed and the resulting developed film is indicative of the state of the organ.

/ J U U yj More recently, another imaging technique has been developed, viz. nuclear magnetic resonance. This avoids the harmful effects sometimes attending X-ray exposure. For improved imaging with X-rays, patients have been given enhancers prior to imaging, either orally or parenterally. After a predetermined time interval for distribution of the enhancer through the patient, the image is taken. To obtain a good image it is desirable that the time after the taking of enhancer be kept to a minimum. On the other hand there is a decrease in effectiveness with time, so desirably the decay should be relatively slow so as to provide a substantial time interval during which imaging can be done. The present invention relates to enhancers for NMR imaging.

In the NMR imaging process protons in the water of the body relax via two mechanisms referred to as T and T . The rate at which the relaxation process occurs may be altered for some water molecules by giving values that contrast with the norm.

Chemicals that enhance NMR images, referred to as contrast agents, are generally paramagnetic in nature. - 3 These may be organic free radicals or transition/lanthanide metals which have from one to seven unpaired electrons.

A necessary prerequisite of any ligand that chelates (binds) a metal to form a contrast agent is that it be stable so as to prevent the loss of the metal and its subsequent accumulation in the body. Other considerations include an ability to reversibly bind water, which in turn increases its contrastability and decreases the dose level required. This ability is clearly important since the interaction between any two nuclear spins through space decreases at a rate equal to the reciprocal of the distance raised to the sixth power.

U.S. Patent 4,647,447 discloses use of an NMR image enhancer consisting of the salt of an anion of a complexing acid and a paramagnetic metal ion. A preferred embodiment is the gadolinium chelate of diethylenetriamine-pentaace tic acid (Gd DTPA). From the data reported therein these appear to perform well. Howeyer, this compound is rapidly excreted by the kidneys, making the timing of the injection extremely critical.

Furthermore, there is virtually no uptake by any solid organ, such as the heart, pancreas or liver.

However, while a number of gadolinium contrast agents are known to work well, there remains the possibility that small amounts of free lanthanides are being released, by decomposition of the agent, into the body. Not being a naturally existing metal in the body, little is known about long term effects.

It is accordingly an object of the present invention to provide, alternative image enhancers which avoid one or more of the aforementioned disadvantages.

It is another object of the invention to provide an NMR-image enhancer which does not release lanthanides into the body.

SUMMARY OF THE INVENTION These and other objects and advantages are realized in accordance with one aspect of the present - 4 invention pursuant to which there is provided the use of a physiologically compatible chelate complex of a chelating compound and a paramagnetic ion of a lanthanide element having an atomic number in the range 57 to 70 or of a transition metal having an atomic number selected from 21 to 29, 42 and 44 and of a non-paramagnetic organic calcium salt for the preparation of a magnetic resonance imaging contrast medium by admixture of said complex and said organic salt.

Advantageously, the chelate complex is of the formula I or II X-CH^ (I) N-A-N or V-CHR1 CHR^-V N(CH2X)3, (II) wherein X is -COOY, -PO-jHY or -CONHOY;.

Y is a. hydrogen atom, a metal ion equivalent or a physiologically biocompatible cation of an inorganic or organic base or amino ac id; A is -CHR -CHR -, -CHn-CH_-(ZC-H--CH-) -, z J z z z z m -c( R.

/A, N(CHX) I CH2-CH2-N(CH2X)2 -CH2-CH-CH2~ or -CH2-CH2-N-CH2-CH2each R} is a hydrogen atom or methyl; R2 and R^ together represent a trimethylene group or a tetramethylene group or individually are hydrogen, C. Q-alkyl, phenyl or benzyl, W is -NN-, -NHCOCH or -NIICS-; - 5 m is the number 1, 2 or 3, is an oxygen atom, a sulfur atom, NCH2X, or NCH CH^, R4 is Cy_8_alky1< V is one of the X groups or is -CF^OK, or -CONH(CH-) X, n n is a number from 1 to 12; if R^, and are hydrogen atoms, both V's together are the group CH X CH X I I -(CH ) -N-CH -CH -N-(CH ) -, w 2 2 2 w w is a number 1, 2 or 3; provided that at least two of the substituents Y are metal ion equivalents of an element with an atomic number of 21 to 29, 42, 44 or 57 to 83.

Alternatively the chelate complex may be a complex of an ion and a ligand, the complexed being an ion of a lanthanide element of atomic numbers 57-70, or of a transition metal of atomic numbers 21-29, 42, or 44; and the ligand being an organic complexing agent which is acyclic or cyclic and contains organic nitrogen, phosphorus, oxygen or sulfur.

In this embodiment, advantageously the complexing agent which forms a ligand is (a) an aminopolycarboxylie acid which is nitrilotriacetic acid, N-hydroxyethy1-N,N1,N'-ethylenediaminetriacetic acid, N,N,N',N”,N-diethylenetriaminepentaacetic acid or N-hydroxyethyliminodiacetic acid; (b) of the formula wherein R and R are identical or different and each is - 6 hydrogen or alkyl of 1-4 carbon atoms and p is an integer of 0-4 ; or (c) an aminopolycarboxylic acid of the formula R, HOOCCH CK.

/CH COOH -(CH_-)-(CH -N-CH -)-(CH ) -t< m 2 2 n 2 m ch2cooh wherein is an integer cf 1 to 4 , is an integer of 0 to 2, andiS C4 -12_alky1, C4_12~alkenyl,C4-12’CyCl° alkyl, ^-cvcloalkeny1, ^2 -hydrocarbo aralkyl, Co n--hydrocarbon alkenyl, CtJ-lz b —12 hydrocarbon aryl or -CH2COOH.

Such complexes are especially useful in the NMR diagnosis of patients to whom they are administered 'followed by imaging.

The acid moiety of the chelate is advantageously carboxy and phosphono, sulpho being less advantageous. The acid groups are joined to the amino nitrogen by an alkyl, i.e. alkylene, radical of up to 4 carbon atoms. Preferably they are acetic acid radicals, i.e. di-carboxymethyl-amino radicals, or phosphonic acid radicals as in U.S. Patent 3,738,937.

Preferably there are two amino groups on adjacent carbon atoms and preferably still they are in the transconfiguration, e.g. trans-N,N,N',N'-tetra-carboxymethy11,2-diaminocyclohexane.

If desired, up to two of the carboxylic acid groups may be reacted to form an amide, a lower alkyl ester and/or an anhydride .

The polyvalent paramagnetic metal may be any of those heretofore used in NMR image enhancement, e.g. iron, chromium, cobalt, europium, terbium, nickel, neodynium, promethium, samarium, , dysprosium, holmium, erbium, thorium, - 7 ytterbium and lutetium. Preferably, however, the metal is iron, manganese, or gadolinium.

The metal containing complex is made by adding the cyclic compound to water and adding four mole equivalents of an alkali such as sodium hydroxide or N-methy1-d-glucamine to dissolve the compound. A 1 molar equivalent of manganese chloride or gadolinium chloride is now introduced into the solution. As a result of the chelate formation, the pH of the solution drops to about 5. When manganese chloride is used, rigorous degassing of all water used and compound formation under an inert nitrogen blanket combine to prevent the formation of oxide products during the course of the reaction. The final pH is adjusted to between 5 and 8 and the solution is passed through a 0.2 micron filter for sterilize tion .

The osmolarity of the resulting solution can be lowered to a physiologically acceptable value by removal of the unnecessary but physiologically acceptable sodium chloride by product. This can be achieved by crystallization, filtering, dialysis or ion exchange.

The superiority of ring-based contrast agents over other contrast agents which have straight alkane chain backbones, e.g. EDTA (ethylene diamine tetraacetic acid) or DTPA (diethylenetriamine pentaacetic acid) apparently resides in the cyclohexane backbone which imparts more rigidity to the molecule and sterically hinders the coordination of water into the nitrogen-metal bond position. While EDTA divalent metal compounds tend to first break the metal nitrogen bonds by water coordination, the instant system loses the oxygen donors first. This is reflected in the proton nuclear magnetic resonance spectrum of the respective molecules. For example, the manganese salt of trans-N,N,N',N'-tetra-carboxymethyl-1,2-diaminocyclohexane (DCTA) has a manganese-nitrogen bond which is considerably more stable than its EDTA analogue. This is reflected in the stability constant (binding ability) towards manganese which is several thousand times better for DCTA than the EDTA chelate. Even though the stability constant of the novel gadolinium complex is approximately the - 8 10 s-owe as the stability constant of Gd DTPA, it is important to note that the novel complex is a tctraacidic ligand while DTPl·. is pentaacidic. Consequently, inner sphere water oordination is greater and the corresponding relaxation values are considerably better. This improvement allows a decrease in dosage and hence a decreased possible toxicity through degradation and release of free gadolinium.

The addition of calcium to the the complexes reduces their toxicity. The calcium should be present in about 0.1 to 200% and preferably about 10 to 100% based on the moles of paramagnetic polyvalent metal. It can be an inorganic salt such as the chloride or sulfate, but organic salts, e.g. the gluconate, lactate, ascorbate, etc., are preferred.

A calcium salt can simply be added to the complex in solution and so administered or the solution can be dried and the dry material later re-dissolved.

The addition of the calcium to the chelate complex surprisingly serves to increase the safety, i.e. to raise the LD^q based on the amount of paramagnetic polyvalent metal present.

For example, the MnEDTP chelate without calcium has an LD^q of 200 umol/kg, a toxic level. The LD^q of the same complex into which 40 mol % of calcium has been incorporated, via calcium gluconate, is in excess of 850 umol/kg, a relatively safe level for human use.

In accordance with another aspect of the invention the acid group is a phosphono moiety. This aspect is applicable even to compounds which are not cyclic, e.g. linear alkylene polyamines such as pcly-nitrogen-substituted phosphono-alky1 alkylenepolyami nes.

As the poly-phosphono alkylated alkylene 35 polyainine there are preferably employed compounds wherein the alkyl and alkylene radicals each contain up to four carbon atoms. The alkylene-polyamine could be diethylenetriamine, for example, but ethylenediamine is preferred. Advantageously the phosphono groups are joined to the nitrogen atoms through a methyl group, i.e. actually a - 9 methylene group. P.acli phosphono group has two acid moieties SO in a compound having lour nitrogen atoms there are eight acid moieties available for complexing.

If desired, up to half of those acid moieties can 5 be bound as salts with non-paramagnetic cations, e.g., alkali metal, alkaline earth metal or ammonium salts, or they may be combined as lower alkyl esters, amides and/or anhydrides. The calcium added as the calcium salt has a beneficial effect even beyond that realized if the acid moieties of the poly-phosphono alkylated alkylene polyamine are already partially in calcium salt form, for example.

One preferred complexing or chelating agent of this type is N,N,N',N'-tetraphosphono-methyl-ethyleneciamine (EDTP) of the structural formula which is commercially available in the form of its sodium salt and free acid.

While lanthanides and particularly gadolinium are highly paramagnetic and useful in accordance with the invention, it is surprising that other less paramagnetic metals perform well, e.g., iron, manganese, copper, cobalt, chromium and nickel.

The complex can be prepared by dissolving a salt of EDTP in water or other solvent and adding a salt of the desired metal, e.g., managanese chloride, in from about half to twice the stoichiometric amount. Additional salts, such as calcium chloride, can be added to tie up additional binding sites in the compound. The solution can then be dialyzed or ιοιί exchanged to remove chloride ions or an - 10 alkali such as NaOH can be added to neutralize the chloride ions, the by-product NaCl being removed or left in solution since it is physiologically acceptable.

The Mn-EDTP complex distributes substantially to 5 the following organs: liver, heart, kidneys, spleen, pancreas, bladder, stomach, small and large intestines.

As noted, manganese is the preferred metal, but other polyvalent paramagnetic metals may be used, e.g., iron, chromium, cobalt, nickel, copper, and the like. The pr c-ferred lanthanide is gadolinium, but others such as lanthanum, cerium, praseodymium, neodymium, promethium, samarium, europium, terbium, dysprosium, holmium, erbium, thulium, ytterbium and lutetium may also be used.

This invention may be used in conjunction with any magnetic resonance machine currently available and is compatible with any of the current known imaging techniques, e.g. a machine such as that of Siemens AG of Erlanger, Federal Republic of Germany.

Further details of imaging systems are described » in the prior art, e.g. NMR A Primer for Medical Imaging by Wolf and Popp Slack Book Division (ISBN 0-943432-19-7) and Scientific American, May 1982, pages 78-88.

The solution of complex may be sterilized and made up into ampules or may be lyophilized into a powder for dissolution when ready to be used. The solution may be mixed with conventional additives such as saline solution, albumin, buffers and the like. If desired, ampules may be made up containing lyophilized powder of the complex in one compartment and a solution of additives in another separated from the first by a frangible barrier. When ready to use, the barrier is broken and the ampule shaken to form a solution suitable for use.

Immediately prior to actual administration of the contrast agent, the reconstituted solution is further oc diluted by addition of a suitable diluent such as: - η Ringer's Injection, USP Sodium Chloride Injection, USP Dextrose Injection, USP (5 percent Dextrose in sterile water) Dextrose Sodium Chloride Injection, USP (5 percent Dextrose in Sodium Chloride) Lactated Rincer's Injection, USP Protein Hydrolysate Injection Low Sodium, USP 5 percent percent with Dextrose 5 percent percent with Invert Sugar 10 percent Water for Injection, USP The manner and dosage of administration and the manner of scanning are substantially the same as in the prior art. With solutions containing about 50 to 500 mmoles of the complex per liter, sufficient solution should be administered orally or parenterally to provide about 1 to 100 umols/kg, corresponding to about 1 to 20 mmol for an adult human patient.For smaller patients or animals, the dosage should be varied accordingly. The particular complex and organ to be imaged will determine the waiting period between administration and imaging.

It will generally be at least about 15 minutes but less than about an hour. During the first few hours the complex is execreted by the liver into the bile.

The invention will be further described in the following illustrative examples wherein all parts are by weight unless otherwise expressed.

Example 1 Synthesis of DCTP (trans-1 , 2-diaininocyclohexane-N , N , N , Ntetramethylenephosphonic acid hydrate). .5 g (0.25 mole) of trans-1,2-diaminocyclohexane and 82 g (1 mole) of phosphorus acid are dissolved - 12 in 140 ml of concentri\ted hydrochloric acid. The solution is heated to reflux (110°C) and 162 g (2.1 moles) of formalin (40% aqueous solution of formaldehyde) are added over the course of 90 minutes. The temperature drops to 94°C and the reaction is maintained at this temperature for hours and then allowed to cool to 25°C overnight. Crystallization is initiated via scratching the walls of the flask. After standing overnight the precipitated product is isolated via filtration and washed with acetone (3 x 100 ml). The DCTP is recrystallized from a minimum of water, isolated by filtration, washed with acetone and air-dried. 64 g (52% yield) of pure product are obtained.

Characterization of DCTP The melting point is 228-232°C (decomposition) with slight darkening observed above 220°C.

The positive ion mass spectrum shows a parent ion at 491 mass units (theoretical: 491). Elemental analysis for DCTP H20 (c y 0H 28N 2° 13P4 } ' Calculated: c, 23.63; H, 5.55; Ν,'5.51; P, 24.38. Found: C, 23.87; H, 5.41; N, 5.48; ?, 24.49. Water, 3.71% by Karl-Fischer titration .

Spectrophotometric complexation analysis of DCTP with standardized copper chloride yields percentages of 100.1, 100.6 and 101.2 (average 100.6) assuming a molecular weight of DCTP.l^O of 508.22.

Nuclear Magnetic Resonance Spectra of DCTP The proton (400.13 MHz), carbon (100.61 MHz) and 3Q phosphorous (161.94 HMz) NMR spectra of trans-1,2-diaminocyclohexane-N, ;i,N,N-tetramethylenephosphonic acid in dimethyl sulfoxide-d6 do not provide structural and peak assignments through standard NMR' techniques. Because of the number of overlapping peaks, 2-dimensional 1H-13C chemical shift correlation NMR techniques are required to make unequivocal peak assignments. The 2D NMR results and analysis of a molecular model indicate an axis of symmetry creating two sets of non-equivalent phosphorous atoms and - 13 diastereotopic protons on the methylene carbons adjacent to the phosphorous atoms. The four methylene units create two sets of chemically non-equivalent nuclei. The NMR peak assignments are as follows: 13C (ppm relative to TMS) : 63.2 (singlet, methine of cyclohexyl) , 50.72 (doublet, Jcp=145.7 Hz, methylene set Λ of phosphonate), :7.10 (doublet, Jcp=140.4 Hz, methylene set B of phosphonate), 23.9 (singlet, beta-methylene of cyclohexyl), 92.9 (singlet, gamma-methylene of eyelohexy1). 1H (ppm Iq relative to TMS): 0.20 (P-OH), 3.55 (methine of eyelohexy1), 3.50, 3.31, 3.27, 2.00 (methylene of phosphonate), 1.72, 1.16 (beta-methylene of cyclohexyl), 2.10, 1.26 (gamma-methylene of cyclohexyl). 31? (ppm relative to H3PO4): -19.2, -1.9.8 The NMR results indicate that the DCTP ligand is relatively rigid on the NMR time-scale; in fact no interconversion is observed up to 60°C. This is in contrast to DCTA, the acetic acid analogue, which is. rapidly interconverting on the NMR time-scale at 25°C.

Example 2 Formation of Calcium Salt of Manganese Complex of DCTA and DCTP 25 a) To 60 ml of degassed water, 1.6 g (0.04 mole) of sodium hydroxide is added. After the alkali is dissolved, 3.6436 g (0.01 mole) of trans-N,N,N',N'-tetracarboxymethyl-1 , 2 diaminocyclohexane monohydrate (Aldrich Chemical Co., Milwaukee, WI) is added to the stirring solution. 1.979 g (0.01 mole) of manganese chloride tetrahydrate is dissolved in 10 ml of degassed water and is added dropwise to the previous solution. After 30 minutes of stirring, 0.1 mole equivalent of calcium chloride is added to the mixture. The pH of the solution is adjusted to 6.5, and water added to bring the final volume to 100 ml, resulting in a final concentration of 100 mM. The clear or faint yellow solution is filtered through a 0.2 - 14 micron filter for sterilization. b) The calcium salt of the manganese complex of trans-1,2-diamino-cyclohexane-N>N,N', N '-tetramethylene phosphonic acid (DCTP) is prepared from the product of Example 1 in a manner analogous to (a). c) Re laxitivities of protons present in water and plasma exposed to the complexes of (a) and (b) (at 10 mHz) (37CC) ·η milliseconds: Table 1 Molar Concentration li T —2 *1 —2 (moles/liter ) Water Water Plasma Plasma (a) (b) (a) (b) (a) (b) (a) (b) 1x10'2 32 16 22 8 25 15 50.5 10 2x 10-3 55 28 43 20 39 34 33.3 27 2 . 5xl0_3 95 54 69 36 74 51 16.9 45 1 . 25xl03 171 88 126 69 121 91 9.7 74 6 . 25xl0~4 . 322 172 223 142 3 . 12x104 599 310 336 212 1 . 56x10“4 971 555 513 269 7 . 30x1 05 1390 987 765 372 d) LD5q values for 40 mice with the complex of (a) : Table 2 Dose(mmole/kg) Sex Fatalities Survivors 30 1 . 5 Male 0 5 1.5 Female 0 5 ·>/ 2.5 Ma le 1 4 2.5 Female 0 5 a 35 4 . 5 Male 2 3 4.5 Female 3 2 5 . 5 Ma le 4 1 5.5 Ferna le 3 2 The LD50 for (a) was determined to be 4.9 mraol/kg with a 95% confidence range between 4.1 and 5.9 mmol/kg. The LD5Q for (b) is much lower at 0.2 mmol/kg. e) Organ distribution of (a) and (b) in male rabbits: The rabbits were sacrificed at 69 minutes post injection for (a) and 15 minutes post-injection for (b) and the proton relaxation values measured in milliseconds, in vitro at 10 mG_, for each of the various organs.

Table 3 Ti ssue Normal Values (a) (b) -2 -i T -2 Brain NA NA 637 82 537 85 Hear t 504 70 367 518 191 40 Lu ng 595 112 4 72 71 323 84 Fat 171 154 176 113 157 95 Skeletal Muse 4 23 47 539 62 395 34 Renal Cortex 338 .85 123 42 109 51 Renal Medulla 672 149 232 71 103 47 Liver 252 64 182/137 28/37 82/66 27/24 Pancreas 464 86 201 49 NA’ NA S toinach 34 9 69 226 52 199 42 Small Intest 352 79 115 4 6 269 60 Large Intest 349 77 219 4 4 248 58 Testis NA NA 623 123 294 79 Urine NA NA 17 11 NA NA NA = Not Available Example 3 Formation of Calcium Salt of Gadolinium Complex of DCTA and DCTP a) 18.218 g (0.05 mole) of trans-N,Ν,Ν ' ,N'-tetracarboxymethyl-1,2 diaininocyclohexane is added to 100 ml of water and 8 g (0.2 mole) of sodium hydroxide is added. 18.585 g (0.05 mole) of gadolinium chloride is then added slowly while stirring. The solution is then stirred for an additional 30 minutes. A 0.1 molar equivalent of calcium chloride is added at this point and the pH of the solution adjusted to 6.5. The volume of the solution is brought to '200 ml. resulting in a final concentration of 250 mM. . The - 16 solution is sterilized by passing through a 0.2 micron filter. b) The calcium salt of the gadolinium complex of trans-i,2-d iamino-eyelohexane-N,N,N’ ,N1 -te trame thylene phosphonic acid is prepared from the product of Example 1 in a manner analogous to (a) . c) Relaxivities of protons present in water and plasma exposed to (a) and (b) at 10 mHz (37 C) in milliseconds: Table 4 Molar Concentration T. Tn T-, Tn —1 -2 -1 -2 (moles /liter) Water Water Plasma Plasma (a) (b) (.a) (b) (a) (b) (a) (b) lxlO-2 22 15 14 8 25 14 20 7 5xl0“3 29 25 25 17 39 20 30 16 2.5xl0~3 55 49 47 35 74 36 59 26 1 . 25xl0~3 104 70 89 65 121 60 10 3 42 6.25xl0~4 183 1 26 161 114 223 95 3 . 12xlO~4 367 257 336 149 1 . 56xl0-4 562 468 513 263 7 . 80xl0-5 983 762 765 447 d) For comparison purposes and to highlight the superior performance of the invention, there follows a table of relaxation values for water and plasma using the N-methyl glucamine salt of Gd DTPA: - 17 Table 5 Molar Concentration Water Plasma moles/liter T, T T, -1 —2 -1 -2 6.25 x 10-3 40 35 39 31 3.13 x 10-3 83 76 69 61 1.56 x 10-3 163 155 134 116 7.81 x 10-4 309 24 0 3.91 x 10-4 582 405 1.95 x 10-4 1015 636 9.77 x 10-5 877 It is noted that the relaxation times in Table 1 with the novel manganese complexes are approximately the same as the gadolinium salts in Table 5, even though Table employs a metal with two less unpaired electrons and which is naturally occurring in the body. The gadolinium salts of this invention in Table 4 are still superior.

Example 4.

Preparation of 100 mM manganese EDTP Complex containing 40 mM calcium. (1) To 300 ml of water containing 0.2 mol of sodium hydroxide, 21.81 g (0.05 mol) of N,N,N',N'-tetraphosphono-methylene-ethylenediamine (referred to as EDTP) is added. The mixture is stirred with a magnetic stirrer until a clear solution is obtained. The pH of the resulting solution is approximately 5.8. (2) 9.90 g (0.05 mol) of manganese chloride u tetrahydrate is dissolved in approximately 15 ml of water and added to the stirring mixture. A precipitate is * developed which dissolves on further stirring. (3) 10 ml. oi 5 M solution of sodium hydroxide is added to the stirring mixture to bring the pH to 5.8. - 18 10 (4) 2.94 g (0.02 mol) of calcium chloride is added to the mixture. A precipitate that develops ssolves after about IS minutes of stirring, and the pH drops to 5 - 6. (5) The pH is brought back to 5.8 with a solution of 5 M sodium hydroxide, (6) The solution is then brought to a final volume of 500 ml resulting in a concentration of 100 mM for the Mn-EDTP complex and 40 mM for calcium. (7) The solution is now filtered through 0.2 urn filters and stored in vials with butyl rubber stoppers.

The solution is then added to water and to human plasma in varying amounts and the relaxivities measured in conventional manner for comparison with those for the gacolmium complex of the 2-N-methylglucamine salt of dicthyle ne-tr iaminepenta-ace tic acid shown in Table 5, supra .

The following results are obtained, low values for both T^ (transverse relaxation mechanism) and T^ (longitudinal relaxation mechanism) being preferred: Table 6 Relaxivity of the compound in water and in human plasma in milliseconds at 10 MHz (37°C). 25 Concentration Water Plasma mol arT1 T 2 h T 2 - 2 1x10 31 19 18 13 - 3 5x10 41 37 3 1 24 - 3 2.5x10 83 74 50 38 - 3 1.25x10 159 123 85 61 6.25x10 ύ’ 298 112 87 - λ 3.125x10 537 160 116 1 . 56x1 0' 884 253 160 7.81xl0~5 1326 353 3 . 9 1 x 1 0'5 478 1.95x10~5 585 9.77xl0~6 653 4.OCxlO-6 797 The relaxivity of the Mn-EDTP-Ca is clearly superior to Gd DTPA. This is especially evident in the T values in plasma. For example, at a concentration of 9.77xl0~6 M, the value for Mn-EDTP-Ca complex is 653 milliseconds; for GdDTPA at a 10-fold higher concentration (9.77x10 5 M) it is 877 msec, i.e., still higher.

E :·: ample 5 .

Pharmacokinetics of the compound of Example 4 in a pure breed beagle dog.

Male dogs are injected with the solution of Example 4 and the comparison compound at 350 umol/kg. Blood is drawn at the indicated times . The plasmas are separated and the T relaxivities in milliseconds measured Table 7 TimeT1T1 min . Mn-EDTP-Ca Gd DTPA Pre-i nj 1102 14 27 10 90 440 20 108 4 44 30 113 551 4 5 153 580 60 222 687 90 404 860 180 777 1282 360 968 Plasma clearance of Gd DTPA is much faster than the Mn-EDTP-Ca Complex. By 180 minutes post-injection, most of the Gd DTPA is cleared from the plasma. Mn-EDTP-Ca is not cleared until 360 minutes post-injection. This gives Mn-EDTP-Ca a larger time window for imaging. - 20 Example 6.

Organ distribution of the compound of Example 4 in male rabbits .

The compound is injected into male rabbits at 50 urnol/kg. The rabbits are sacrificed at 15 minutes post injection and the T relaxivity of internal organs measured in vitro at 5 MHz (milliseconds) . The results are as follows : Table 3 Organ T,Ti Mn-Ef)TP-Ca normil · Heart 240 482 Lung 413 585 Fat 161 180 Skeletal Muscle 260 411 Renal Coster 101 342 Renal Medulla 77 782 Liver 43 260 Spleen 200 473 Pancreas 146 265 Bladder 199 511 S tomach 1 30 305 Small Intestine 155 317 Large Intestine 133 328 By comparison according to Amer. J .Roentol. 14 3, 1226, the distribution of Gd DTPA in man at 30 minutes post-injection in milliseconds is: Table 9 Organ Pre T1 Post T1 Fa t 220 185 Muscle 460 335 Liver 350 195 Spleen 560 285 Kidneys 820 205 The organ distribution pattern of Mn-EDTP-Ca is substantially different from Gd-DTPA. It enters the hepatobiliary system resulting in a substantial decrease in - 21 Τι values of the liver, spleen, pancreas, and small and large intestines. Gd DTPA, being a vascular agent, is mainly cleared by the kidneys and does not substantially interact with the hepatobiliary system. Mn-EDTP-Ca also distributes'to the heart. EKG studies indicate that it does not disturb the function of the heart.

Example 7.

To 10 ml of water containing 5 ml of 1 N sodium hydroxide is added 2.0 g (5 mmoles) of 1,4,7,10-tetraazacyclododecane - N,N',N'',N'''-tetraacetic acid. 1.3 g (5 mmoles) of GdCl^ is added and the suspension heated to 50°C for 2 hours. Calcium chloride (1 mmole) is added and the pH of the solution adjusted with 1 N sodium hydroxide to 6.5. The clear solution is filtered through a 0.2 micron filter for sterilization.· Example 8.

To 100 ml of water containing 10 g (100 mmoles) of N-methylglucamine is added 19.7 g (50 mmoles) of diethylene-triamine-N,N' ,N‘ ' ,N'' '-pentaacetic acid. 13 g (50 mmoles) of GdCl^ is added and the slurry stirred for 1 hour at room temperature. Calcium ascorbate (3.9 g, 10 mmoles) is added and the pH adjusted to 6.5 with 1 N sodium hydroxide. The clear 500 mM solution is filtered through a 0.2 micron filter for sterilization prior to use.

It will be understood that the specification and examples are illustrative but not limitative of the present invention and that other embodiments within the spirit and scope of the invention will suggest themselves to those skilled in the art.

Claims (5)

Claims

1. The use of a physiologically compatible chelate complex of a chelating compound and a paramagnetic ion of a lanthanide element having an atomic number in the range 57 to 70 or of a transition metal having an atomic number selected from 21 to 29, 42 and 44 and of a nonparamagnetic organic calcium salt for the preparation of a magnetic resonance imaging contrast medium by admixture of said complex and said organic salt.

2. Use as claimed in claim 1 wherein said paramagnetic metal ion is an ion of Fe, Mn or Gd.

3. Use as claimed in either of claims 1 and 2 wherein said chelating compound is selected from EDTP, DCTP, DCTA, 1,4,7, lO-tetraazacyciododecane-Ν,Ν' ,N,N ' tetracetic acid and DTPA.

4. Use as claimed in any one of claims 1 to 3 wherein said organic salt is selected from calcium gluconate, calcium lactate and calcium ascorbate.

5. Use as claimed in claim 1 substantially as described herein with reference to the Examples.