USE OF MITOXANTRONE PREPARATION IN PREPARATION OF DRUG FOR DIAGNOSING AND TREATING BREAST CANCER

Abstract

The use of a mitoxantrone preparation in the preparation of a drug for diagnosing and treating breast cancer. Provided is the use of mitoxantrone and/or a pharmaceutically acceptable salt thereof in the preparation of a lymphatic tracer in a disease associated with breast resection. No local or systemic toxic and side effects are seen after local injection of the preparation, suggesting that the preparation has good tolerance, effectiveness and safety, which provides a new treatment idea for thoroughly curing breast cancer in a breast cancer patient.

Claims

1. Use of mitoxantrone and/or a pharmaceutically acceptable salt thereof in preparation of a lymphatic tracer for a disease related to mastectomy.

2. A lymphatic tracing method for a disease related to mastectomy, comprising: administering mitoxantrone and/or a pharmaceutically acceptable salt thereof to a patient, the mitoxantrone and/or the pharmaceutically acceptable salt thereof being used as a lymphatic tracer.

3. The method according to 2, wherein the disease related to mastectomy is selected from breast tumor, breast cyst, breast fibroma, and breast tuberculosis.

4. The method according to claim 2, wherein the breast tumor comprises benign breast tumor and malignant breast tumor, preferably, the malignant breast tumor is breast cancer; and preferably, the lymphatic tracer is used for tracing the lymph in a breast cancer.

5. The method according to claim 2, wherein the lymphatic tracer contains the mitoxantrone and/or the pharmaceutically acceptable salt thereof and a pharmaceutically acceptable excipient, preferably, the pharmaceutically acceptable excipient comprises, but is not limited to, a buffer, a carrier, a stabilizer, or a preservative; preferably, the lymphatic tracer is an injection; preferably, the injection is in a form of solution, lyophilized powder, emulsion, liposome, nanoparticles, nanocrystals, microcrystals, microspheres or gel; and preferably, the injection in the form of solution is a sodium chloride injection or a glucose injection.

6. The method according to claim 2, wherein the injection is administered subcutaneously, intramuscularly or subserosally, and preferably, subcutaneously or subserosallly; preferably, the injection is administered locally; preferably, the injecting sites are on the breast gland and/or tissues and organs around the breast; preferably, the injection is administered at multiple sites; preferably, the concentration of the injection is 2-10 mg/mL; and preferably, the volume of the injection is 0.1-3.0 mL, and more preferably, at least 0.1 mL of the injection at a concentration of 5 mg/mL is administered; and preferably, a total dosage does not exceed 3.0 mL.

7. The method according to claim 2, wherein the pharmaceutically acceptable salt is a pharmaceutically acceptable salt formed by the mitoxantrone and an inorganic acid or an organic acid, preferably, the inorganic acid is, for example, hydrochloric acid, hydrobromic acid, sulfuric acid, nitric acid, carbonic acid or phosphoric acid; preferably, the organic acid is selected from aliphatic, cycloaliphatic, aromatic, araliphatic, heterocyclic, carboxylic, and sulfonic organic acids, such as formic acid, acetic acid, propionic acid, glycolic acid, gluconic acid, lactic acid, pyruvic acid, oxalic acid, malic acid, maleic acid, malonic acid, succinic acid, fumaric acid, tartaric acid, citric acid, aspartic acid, ascorbic acid, glutamic acid, anthranilic acid, benzoic acid, cinnamic acid, mandelic acid, pamoic acid, phenylacetic acid, methanesulfonic acid (methanesulfonate), ethanesulfonic acid, p-toluenesulfonic acid, and salicylic acid; and preferably, the pharmaceutically acceptable salt is selected from mitoxantrone hydrochloride, mitoxantrone oxalate, mitoxantrone sulfate, mitoxantrone phosphate, mitoxantrone acetate, and mitoxantrone citrate; and more preferably, the pharmaceutically acceptable salt is mitoxantrone hydrochloride.

8. The method according to claim 2, wherein the lymphatic tracer contains a pH regulator, preferably, the pH regulator is one or more selected from the group consisting of hydrochloric acid, phosphoric acid, sulfuric acid, oxalic acid, acetic acid, and citric acid.

9. The method according to claim 2, wherein the lymphatic tracer contains an antioxidant, preferably, the antioxidant is one or more selected from the group consisting of sodium sulfite, sodium bisulfite, sodium pyrosulfite, sodium thiosulfate, and disodium edetate, and preferably, the antioxidant is sodium pyrosulfite or disodium edetate; preferably, the lymphatic tracer contains the mitoxantrone or the salt thereof, sodium chloride, acetic acid, sodium acetate, and sodium pyrosulfite, and more preferably, the lymphatic tracer further contains sodium sulfate; preferably, the lymphatic tracer contains the mitoxantrone or the salt thereof, sodium chloride, acetic acid, sodium acetate, and disodium edetate; preferably, a pH value of the injection is in a range of 2.8-4.3; preferably, the content of the mitoxantrone or mitoxantrone in the salt thereof is 1-15 mg/mL, preferably, 2-10 mg/mL, and more preferably, 2 mg/mL, 5 mg/mL or 10 mg/mL, in terms of weight by volume; preferably, the content of the sodium chloride is 3-18 mg/mL, preferably, 4-16 mg/mL, and more preferably, 4 mg/mL, 8 mg/mL or 16 mg/mL, in terms of weight by volume; preferably, the content of the acetic acid is 0.15-1 mg/mL, preferably, 0.23-0.92 mg/mL, and more preferably, 0.23 mg/mL, 0.46 mg/mL or 0.92 mg/mL, in terms of weight by volume; preferably, the content of the sodium acetate is 0.03-0.15 mg/mL, preferably, 0.05-0.1 mg/mL, and more preferably, 0.05 mg/mL or 0.1 mg/mL, in terms of weight by volume; preferably, the content of the antioxidant is 0.05-0.3 mg/mL, preferably, 0.8-0.12 mg/mL, and more preferably, 0.1 mg/mL, 0.2 mg/mL or 0.3 mg/mL, in terms of weight by volume; and preferably, the content of the sodium sulfate is 0.05-0.6 mg/mL, preferably, 0.15-0.45 mg/mL, and more preferably, 0.15 mg/mL, 0.3 mg/mL or 0.45 mg/mL, in terms of weight by volume.

10. The method according to claim 2, wherein the injection is prepared by the following method: (1) weighing prescribed amounts of acetic acid, sodium acetate, sodium chloride, and disodium edetate, or weighing prescribed amounts of acetic acid, sodium acetate, sodium chloride, and sodium pyrosulfite, or weighing prescribed amounts of acetic acid, sodium acetate, sodium chloride, sodium pyrosulfite, and sodium sulfate, mixing them with a solvent, and dissolving them to obtain a mixed solution of excipients, preferably, the solvent being water for injecting, preferably, the excipients being dissolved by stirring; and (2) mixing the mixed solution of excipients obtained in the step (1) with prescribed amounts of mitoxantrone and/or a pharmaceutically acceptable salt thereof, preferably, the mitoxantrone and/or the pharmaceutically acceptable salt thereof being dissolved by stirring, preferably, the mitoxantrone and/or the pharmaceutically acceptable salt thereof being dissolved by stirring for 10-30 min; preferably, the method further comprises the following step: (3) filtering, preferably, filtering with 0.45 .Math.m and/or 0.22 .Math.m of filter membranes; preferably, the method further comprises the following step: (4) bottling and filling with nitrogen gas, preferably, sterilization being performed at 121° C. for 15 min after filling with nitrogen gas; preferably, a pH value of the injection is in a range of 2.8-4.3; and preferably, the injection is prepared into a specification of 2 mL:10 mg.

Description

DETAILED DESCRIPTION OF EMBODIMENTS

[0067] For purposes of clarity and conciseness of description, features are described herein as part of the same or separate embodiments. However, it is to be understood that the scope of the present disclosure may include some embodiments having combinations of all or some of the described features.

Example 1 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 1

[0068] TABLE-US-00001 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 11.64 0.582 sodium chloride 16.0 0.8 acetic acid 0.92 0.046 sodium acetate 0.10 0.005 disodium edetate 0.40 0.02 water for injecting (made up to) 2,000 mL —

[0069] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, and disodium edetate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.5.

Example 2 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 2

[0070] TABLE-US-00002 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 23.28 1.164 sodium chloride 32.0 1.6 acetic acid 1.84 0.092 sodium acetate 0.20 0.01 sodium pyrosulfite 0.40 0.02 sodium sulfate 0.60 0.03 water for injecting (made up to) 2,000 mL —

[0071] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, sodium pyrosulfite, and sodium sulfate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.4.

Example 3 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 3

[0072] TABLE-US-00003 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 2.91 0.1455 sodium chloride 16.0 0.8 acetic acid 0.92 0.046 sodium acetate 0.10 0.005 disodium edetate 0.40 0.02 water for injecting (made up to) 2,000 mL —

[0073] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, and disodium edetate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.6.

Example 4 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 4

[0074] TABLE-US-00004 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 11.64 0.582 sodium chloride 16.0 0.8 acetic acid 0.92 0.046 sodium acetate 0.10 0.005 sodium pyrosulfite 0.20 0.01 sodium sulfate 0.30 0.015 water for injecting (made up to) 2,000 mL —

[0075] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, sodium pyrosulfite, and sodium sulfate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.7.

Example 5 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 5

[0076] TABLE-US-00005 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 23.28 1.164 sodium chloride 16.0 0.8 acetic acid 0.92 0.046 sodium acetate 0.10 0.005 sodium pyrosulfite 0.40 0.020 sodium sulfate 0.90 0.045 water for injecting (made up to) 2,000 mL —

[0077] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, sodium pyrosulfite, and sodium sulfate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.6.

Example 6 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 6

[0078] TABLE-US-00006 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 23.28 1.164 sodium chloride 16.0 0.8 acetic acid 0.92 0.046 sodium acetate 0.10 0.005 disodium edetate 0.60 0.03 water for injecting (made up to) 2,000 mL —

[0079] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, and disodium edetate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.7.

Example 7 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 7

[0080] TABLE-US-00007 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 11.64 0.582 sodium chloride 8.0 0.4 acetic acid 0.46 0.023 sodium acetate 0.10 0.005 sodium pyrosulfite 0.40 0.020 water for injecting (made up to) 2,000 mL —

[0081] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, and sodium pyrosulfite were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.9.

Example 8 Preparation of a Mitoxantrone Hydrochloride Injection According to Formula 8

[0082] TABLE-US-00008 Raw materials and excipients Usage amount g % mitoxantrone hydrochloride 5.82 0.291 sodium chloride 8.0 0.4 acetic acid 0.46 0.023 sodium acetate 0.10 0.005 sodium pyrosulfite 0.40 0.020 sodium sulfate 0.60 0.03 water for injecting (made up to) 2,000 mL —

[0083] Prescribed amounts of sodium chloride, acetic acid, sodium acetate, sodium pyrosulfite, and sodium sulfate were weighed, added into a prescribed amount of water for injecting, and dissolved by stirring; a prescribed amount of mitoxantrone hydrochloride was added after the excipients were dissolved, and dissolved by stirring for 30 min; and the mixed solution was finely filtered with 0.45 .Math.m and 0.22 .Math.m of filter membranes, bottled and filled with nitrogen gas, capped, and sterilized at 121° C. for 15 min. A pH value of the mitoxantrone hydrochloride injection was detected to be 3.5.

Example 9 Studies on Pharmacokinetic and Pharmacodynamic Assay of a Mitoxantrone Hydrochloride Injection

[0084] A target organ of a mitoxantrone hydrochloride injection for lymphatic tracing is a lymph node in the breast drainage area. When mitoxantrone hydrochloride is compounded with hydrochloric acid, a uniform acidic solution can be formed. After a mitoxantrone hydrochloride injection is administered to the tissues space, the pH of the microenvironment changes, and mitoxantrone hydrochloride will gradually precipitate into nanocrystals. The crystals prevent mitoxantrone hydrochloride from entering the blood circulation through capillaries. Due to high permeability of lymphatic capillaries, mitoxantrone hydrochloride can enter the lymphatic capillaries through endothelial cell space as well as pinocytosis and phagocytosis of endothelial cells, reach regional lymph nodes through lymphatic drainage and enrich in regional lymph nodes, and stay in the lymph nodes for a period of time, thereby achieving effects of staining and tracing of the lymph nodes.

[0085] In order to test the safety and efficacy of a mitoxantrone hydrochloride injection for lymphatic tracing in tracing of lesion-draining lymph nodes in a patient with breast cancer, and to test the tolerance and in vivo pharmacokinetics of the mitoxantrone hydrochloride injection for lymphatic tracing in the subject with breast cancer so as to determine a safe dose range, this example adopted a single-center, randomized, open, and blank-controlled trial design. After the breast was fully exposed, a mitoxantrone hydrochloride injection for lymphatic tracing at a concentration of 5 mg/mL was administered at multiple sites on the breast gland. According to the size of the breast, a total dose of the injection was 0.1-3.0 mL. The tolerance in human being and pharmacokinetics in subjects were tested group by group, and the efficacy of the investigational drug was observed at the same time.

[0086] Pharmacokinetic results: the mitoxantrone hydrochloride injection is rapidly absorbed after being peritumorally administered, and the peak is basically reached 15-30 min after injecting. Moreover, the drug is metabolized rapidly after entering the blood, and the drug in the plasma is almost completely metabolized 60 min, 120 min at most, after the administration. In addition, the plasma concentration after the administration generally shows a dose-dependent trend, plasma concentrations in different subjects in a low-dose group are all lower than the lower limit of quantification at various time points; plasma concentrations in various patients in medium- and high-dose groups are equal to or higher than the lower limit of quantification at up to 4 time points; and the detected maximum concentration is 79.4 ng/mL only, which is about 6.5 times lower than the maximum concentration of 510±206 ng/mL reported in a document for patients with acute leukemia having received mitoxantrone chemotherapy by infusion administration (10-12 mg/m.sup.2/d). In the document, high-dose mitoxantrone chemotherapy is used for treating ovarian cancer, the maximum tolerated total dosage of mitoxantrone administered by intravenous bolus is 75 mg/m.sup.2, and AUC at this dose is 560-1700 ng×h/mL, which is 10.7-32.5 times the maximum AUC (3143 ng × min/ml) in the present trial.

Example 10 Application of a Mitoxantrone Hydrochloride Injection for Lymphatic Tracing in an Operation for a Patient with Beast Cancer

1. Clinical Trial Design

[0087] The trial adopted a single-center, positive, and self-controlled trial design. According to the principle of dose escalation, the tolerance and pharmacokinetics in subjects were tested by intraoperative injection group by group, and the efficacy of the investigational drug was observed at the same time. The trial was planned to select 12 to 24 patients with breast cancer. The patients were divided into 4 groups with 3-6 patients in each group, and 0.5 mL, 1.0 mL, 2.0 mL, and 3.0 mL of mitoxantrone hydrochloride injection at a concentration of 5 mg/mL were respectively administered to each patient in the groups. One breast of each subject was injected with 2 mCi of nuclide-labeled sulfur colloid into the glands around the tumor 12 to 24 h before the operation in the nuclear medicine department, and imaging data was obtained to determine positions and the number of SLNs. The other breast of each subject was injected with the mitoxantrone hydrochloride injection, and each subject received only one dose of the investigational drug. The safety of the investigational drug was observed, the optimal dose and use method of the investigational drug were explored, and the efficacy of the investigational drug was investigated at the same time.

[0088] Investigational drug: the mitoxantrone hydrochloride injection for lymphatic tracing was injected into the glands around the tumor with a skin test needle in the operation, and the injecting sites were the same as those of the contrast drug, and a total dosage was 0.5-3.0 mL. Contrast drug: each subject participating in the trial was injected with 2 mCi of nuclide-labeled sulfur colloid into the glands around the tumor 12-24 h before the operation in the nuclear medicine department.

[0089] The trial was planned to select 9-18 18-70-year-old female subjects with breast cancer. Actually, 10 subjects completed the trial. [0090] Efficacy evaluation [0091] Primary endpoint [0092] Comparison of success rates of SLN tracing with the investigational drug and the contrast drug [0093] Success rate of SLN tracing = the total number of patients with successful SLN tracing/the total number of patients participating in a trial × 100% [0094] The successful SLN tracing with the investigational drug refers to that SLNs traced by the investigational drug are stained axillary lymph nodes and lymph nodes to which stained lymph vessels point.

[0095] The successful SLN tracing with the contrast drug refers to that SLNs recognized by the contrast (nuclide) tracer are lymph nodes with the maximum Gamma probe count and a count value 10 times or more than the background count.

[0096] Secondary endpoint

[0097] The number of SLNs traced by the investigational drug and the contrast drug, the number of SLNs traced together by the two tracers, and the number of SLNs that were not traced by the two drugs but clinically suspected were recorded.

[0098] Pathological states of SLNs detected by the investigational drug or the contrast drug were recorded.

[0099] The local damage caused by the investigational drug or the contrast drug was recorded.

[0100] Safety and tolerance evaluations

[0101] All subjects using the investigational drug were included in the evaluation of safety, tolerance, and endpoint indicators. The safety evaluation of the clinical trial was carried out until 21±3 days after the operation was completed. The evaluation was carried out by comparing hospital examination results two weeks before the trial to postoperative laboratory test results according to the adverse event evaluation basis, i.e., NCI’s Criteria for Adverse Events Version 4.03 (CTCAE 4.0.3). The relationship between grades of adverse events and the investigational drug was judged to determine the maximum tolerated dose and a safe dose range.

2. Efficacy Results of the Clinical Trial

[0102] The study shows that the success rate of SLN tracing with the mitoxantrone hydrochloride injection for lymphatic tracing is higher, and there is no significant difference between the mitoxantrone hydrochloride injection and the contrast nuclide-labeled sulfur colloid. The success rates of SLN tracing with the contrast drug and groups of the investigational drug at a dose of 0.5 mL or 2.0 mL are all 100%. However, the success rates of SLN tracing with the contrast drug and a group of the investigational drug at a dose of 1.0 mL are 75%, and by analyzing the subjects participating in the trial, macro-cancerometastasis is found in 1 subject in this dose group. The reason may be that a lesion is large enough to block lymph vessels, and lymph nodes detected by both of the investigational drug and the contrast drug are not traced, causing failed tracing in the subject. There is no significant difference between the number of SLNs traced by the investigational drug at each dose and the number of SLNs traced by the contrast drug, as well as the number of SLNs traced together by the two tracers. There is no significant difference between the number of SLNs that are not traced by the investigational drug at each dose but clinically suspected and the number of SLNs that are not traced by the contrast drug but clinically suspected. It was indicated that compared with the nuclide method, the test drug has a good lymph node tracing effect. Pathological results of SLNs detected by the investigational drug and the contrast drug show that no cancerometastasis is found in SLNs traced by the investigational drug and the contrast drug.

Example 11 Application Case of a Mitoxantrone Hydrochloride Injection for Lymphatic Tracing in a Patient with Left Breast Cancer

[0103] Preoperative diagnosis: right breast cancer (cT1N0M0) [0104] Postoperative diagnosis: right breast cancer (sT1N0M0) [0105] Operation name: total mastectomy for right breast + SLN labelling + effusion drainage × 2 [0106] Intraoperative findings: when the right axilla is explored, six intumescent lymph nodes are seen, among which lymph nodes A, B, C, and D are stained blue and have nuclides, and lymph nodes E and F are not stained blue and do not have nuclides.

[0107] Operative procedures are as follows. The patient was placed in the supine position with the right upper limb abducing. After the general anesthesia took effect, 1.5 mL of drug at a concentration of 2 mL: 10 mg was injected at 4 sites around the tumor, and the surgery field was conventionally disinfected and draped. Preoperative biopsy results of the patient showed a clear diagnosis of right breast cancer. A transverse incision with a length of about 10.0 cm was formed on the right chest wall, the skin flap was dissociated up to the subclavian area, down to the costal arch, laterally to the posterior axillary line, and medially to the midline. The right entire breast, the surrounding adipose tissue, and the pectoralis major fascia were cut and removed. When the right axilla was explored, six intumescent lymph nodes were seen, among which lymph nodes A, B, C, and D were stained blue and had nuclides, and lymph nodes E and F were not stained blue and did not have nuclides. The lymph nodes were subjected to frozen pathology examination, and a pathological report (right breast SLNs A, B, C, D, E, and F) was obtained after 30 min and showed that no cancerometastasis was found in frozen lymph node slices. The wound was rinsed, after no active bleeding was found, the numbers of instruments and gauzes were checked, one drain was respectively placed at the axilla and the chest wall, and the incision was sutured. The operation was completed smoothly, anesthesia was appropriate, and the patient was transferred to the ward after operation.

[0108] Pathological examination results: (right breast SLNs A, B, C, D, E, and F) no cancerometastasis is found in frozen lymph node slices.

[0109] A total of 6 lymph nodes are detected, among which 4 lymph nodes are stained.